Your search keyword '"Lee R. Haines"' showing total 60 results

1. Establishment and partial characterisation of a new cell line derived from adult tissues of the tsetse fly Glossina morsitans morsitans

Author

Lesley Bell-Sakyi, Lee R. Haines, Giovanni Petrucci, Alexandra Beliavskaia, Catherine Hartley, Jing Jing Khoo, Benjamin L. Makepeace, Adly M. M. Abd-Alla, and Alistair C. Darby

Subjects

insect, cell line, tsetse, Glossina morsitans morsitans, iflavirus, negevirus, Wolbachia, Infectious and parasitic diseases, RC109-216

Abstract

Abstract Background Insect cell lines play a vital role in many aspects of research on disease vectors and agricultural pests. The tsetse fly Glossina morsitans morsitans is an important vector of salivarian trypanosomes in sub-Saharan Africa and, as such, is a major constraint on human health and agricultural development in the region. Methods Here, we report establishment and partial characterisation of a cell line, GMA/LULS61, derived from tissues of adult female G. m. morsitans. GMA/LULS61 cells, grown at 28 °C in L-15 (Leibovitz) medium supplemented with foetal bovine serum and tryptose phosphate broth, have been taken through 23 passages to date and can be split 1:1 at 2-week intervals. Karyotyping at passage 17 revealed a predominantly haploid chromosome complement. Species origin and absence of contaminating bacteria were confirmed by PCR amplification and sequencing of fragments of the COI gene and pan-bacterial 16S rRNA gene respectively. However, PCR screening of RNA extracted from GMA/LULS61 cells confirmed presence of the recently described Glossina morsitans morsitans iflavirus and Glossina morsitans morsitans negevirus, but absence of Glossina pallipides salivary gland hypertrophy virus. GMA/LULS61 cells supported infection and growth of 6/7 different insect-derived strains of the intracellular bacterial symbiont Wolbachia. Conclusions The GMA/LULS61 cell line has potential for application in a variety of studies investigating the biology of G. m. morsitans and its associated pathogenic and symbiotic microorganisms. Graphical Abstract

Published

2024

2. Gastrointestinal parasites in captive olive baboons in a UK safari park

Author

Alexandra Juhasz, Elly Spiers, Ellie Tinsley, Emma Chapman, William Shaw, Marion Head, Lucas J. Cunningham, John Archer, Sam Jones, Lee R. Haines, Naomi Davies Walsh, Bridget Johnson, Jen Quayle, Jayne Jones, Elwyn James LaCourse, Jonathan Cracknell, John Russell Stothard, Rudi Cassini, and Laura Rinaldi

Subjects

giardiasis, Papio anubis, strongyloidiasis, Strongyloides fuelleborni, trichuriasis, Trichuris trichiura, Biochemistry, QD415-436, Infectious and parasitic diseases, RC109-216, Microbiology, QR1-502

Abstract

From the safety inside vehicles, Knowsley Safari offers visitors a close-up encounter with captive olive baboons. As exiting vehicles may be contaminated with baboon stool, a comprehensive coprological inspection was conducted to address public health concerns. Baboon stools were obtained from vehicles, and sleeping areas, inclusive of video analysis of baboon–vehicle interactions. A purposely selected 4-day sampling period enabled comparative inspections of 2662 vehicles, with a total of 669 baboon stools examined (371 from vehicles and 298 from sleeping areas). As informed by our pilot study, front-line diagnostic methods were: QUIK-CHEK rapid diagnostic test (RDT) (Giardia and Cryptosporidium), Kato–Katz coproscopy (Trichuris) and charcoal culture (Strongyloides). Some 13.9% of vehicles were contaminated with baboon stool. Prevalence of giardiasis was 37.4% while cryptosporidiosis was

Published

2023

3. Investigating the unaccounted ones: insights on age-dependent reproductive loss in a viviparous fly

Author

Sinead English, Antoine M. G. Barreaux, Robert Leyland, Jennifer S. Lord, John W. Hargrove, Glyn A. Vale, and Lee R. Haines

Subjects

tsetse, pregnancy loss, prenatal mortality, reproductive senescence, offspring quality, Evolution, QH359-425, Ecology, QH540-549.5

Abstract

Most empirical and theoretical studies on reproductive senescence focus on observable attributes of offspring produced, such as size or postnatal survival. While harder to study, an important outcome of reproduction for a breeding individual is whether a viable offspring is produced at all. While prenatal mortality can sometimes be directly observed, this can also be indicated through an increase in the interval between offspring production. Both direct reproductive loss and presumed losses have been found to increase in older females across several species. Here, we study such reproductive loss (or “abortion”) in tsetse, a viviparous and relatively long-lived fly with high maternal allocation. We consider how age-dependent patterns of abortion depend on the developmental stage of offspring and find that, as per previous laboratory studies, older females have higher rates of abortion at the late-larval stage, while egg-stage abortions are high both for very young and older females. We track the reproductive output of individual females and find little evidence that experiencing an abortion is an adaptive strategy to improve future reproductive outcomes. After an abortion, females do not generally take less time to produce their next offspring, these offspring are not larger, and there is no sex bias towards females, the sex with presumed higher fitness returns (being slightly larger and longer-lived than males, and with high insemination rates). Abortion rates are higher for breeding females experiencing stress, measured as nutritional deprivation, which echoes previous work in tsetse and other viviparous species, i.e., humans and baboons. We discuss our results in the context of studies on reproductive loss across taxa and argue that this is an important yet often overlooked reproductive trait which can vary with maternal age and can also depend on environmental stressors.

Published

2023

4. Oxidative Phosphorylation Is Required for Powering Motility and Development of the Sleeping Sickness Parasite Trypanosoma brucei in the Tsetse Fly Vector

Author

Caroline E. Dewar, Aitor Casas-Sanchez, Constentin Dieme, Aline Crouzols, Lee R. Haines, Álvaro Acosta-Serrano, Brice Rotureau, and Achim Schnaufer

Subjects

ATP synthase, Trypanosoma brucei, human African trypanosomiasis, mitochondria, mitochondrial metabolism, oxidative phosphorylation, Microbiology, QR1-502

Abstract

ABSTRACT The single-celled parasite Trypanosoma brucei is transmitted by hematophagous tsetse flies. Life cycle progression from mammalian bloodstream form to tsetse midgut form and, subsequently, infective salivary gland form depends on complex developmental steps and migration within different fly tissues. As the parasite colonizes the glucose-poor insect midgut, ATP production is thought to depend on activation of mitochondrial amino acid catabolism via oxidative phosphorylation (OXPHOS). This process involves respiratory chain complexes and F1Fo-ATP synthase and requires protein subunits of these complexes that are encoded in the parasite's mitochondrial DNA (kDNA). Here, we show that progressive loss of kDNA-encoded functions correlates with a decreasing ability to initiate and complete development in the tsetse. First, parasites with a mutated F1Fo-ATP synthase with reduced capacity for OXPHOS can initiate differentiation from bloodstream to insect form, but they are unable to proliferate in vitro. Unexpectedly, these cells can still colonize the tsetse midgut. However, these parasites exhibit a motility defect and are severely impaired in colonizing or migrating to subsequent tsetse tissues. Second, parasites with a fully disrupted F1Fo-ATP synthase complex that is completely unable to produce ATP by OXPHOS can still differentiate to the first insect stage in vitro but die within a few days and cannot establish a midgut infection in vivo. Third, parasites lacking kDNA entirely can initiate differentiation but die soon after. Together, these scenarios suggest that efficient ATP production via OXPHOS is not essential for initial colonization of the tsetse vector but is required to power trypanosome migration within the fly. IMPORTANCE African trypanosomes cause disease in humans and their livestock and are transmitted by tsetse flies. The insect ingests these parasites with its blood meal, but to be transmitted to another mammal, the trypanosome must undergo complex development within the tsetse fly and migrate from the insect's gut to its salivary glands. Crucially, the parasite must switch from a sugar-based diet while in the mammal to a diet based primarily on amino acids when it develops in the insect. Here, we show that efficient energy production by an organelle called the mitochondrion is critical for the trypanosome's ability to swim and to migrate through the tsetse fly. Surprisingly, trypanosomes with impaired mitochondrial energy production are only mildly compromised in their ability to colonize the tsetse fly midgut. Our study adds a new perspective to the emerging view that infection of tsetse flies by trypanosomes is more complex than previously thought.

Published

2022

5. Isolation in Natural Host Cell Lines of Wolbachia Strains wPip from the Mosquito Culex pipiens and wPap from the Sand Fly Phlebotomus papatasi

Author

Lesley Bell-Sakyi, Alexandra Beliavskaia, Catherine S. Hartley, Laura Jones, Lisa Luu, Lee R. Haines, James G. C. Hamilton, Alistair C. Darby, and Benjamin L. Makepeace

Subjects

mosquito, sand fly, tick cell line, Wolbachia, Culex pipiens, Phlebotomus papatasi, Science

Abstract

Endosymbiotic intracellular bacteria of the genus Wolbachia are harboured by many species of invertebrates. They display a wide range of developmental, metabolic and nutritional interactions with their hosts and may impact the transmission of arboviruses and protozoan parasites. Wolbachia have occasionally been isolated during insect cell line generation. Here, we report the isolation of two strains of Wolbachia, wPip and wPap, during cell line generation from their respective hosts, the mosquito Culex pipiens and the sand fly Phlebotomus papatasi. wPip was pathogenic for both new C. pipiens cell lines, CPE/LULS50 and CLP/LULS56, requiring tetracycline treatment to rescue the lines. In contrast, wPap was tolerated by the P. papatasi cell line PPL/LULS49, although tetracycline treatment was applied to generate a Wolbachia-free subline. Both Wolbachia strains were infective for a panel of heterologous insect and tick cell lines, including two novel lines generated from the sand fly Lutzomyia longipalpis, LLE/LULS45 and LLL/LULS52. In all cases, wPip was more pathogenic for the host cells than wPap. These newly isolated Wolbachia strains, and the novel mosquito and sand fly cell lines reported here, will add to the resources available for research on host–endosymbiont relationships, as well as on C. pipiens, P. papatasi, L. longipalpis and the pathogens that they transmit.

Published

2021

6. An Intranuclear Sodalis-Like Symbiont and Spiroplasma Coinfect the Carrot Psyllid, Bactericera trigonica (Hemiptera, Psylloidea)

Author

Saptarshi Ghosh, Noa Sela, Svetlana Kontsedalov, Galina Lebedev, Lee R. Haines, and Murad Ghanim

Subjects

psyllid, Bactericera trigonica, Candidatus Liberibacter solanacearum, secondary endosymbiont, Sodalis, Spiroplasma, Biology (General), QH301-705.5

Abstract

Endosymbionts harbored inside insects play critical roles in the biology of their insect host and can influence the transmission of pathogens by insect vectors. Bactericera trigonica infests umbelliferous plants and transmits the bacterial plant pathogen Candidatus Liberibacter solanacearum (CLso), causing carrot yellows disease. To characterize the bacterial diversity of B. trigonica, as a first step, we used PCR-restriction fragment length polymorphism (PCR-RFLP) and denaturing gradient gel electrophoresis (DGGE) analyses of 16S rDNA to identify Sodalis and Spiroplasma endosymbionts. The prevalence of both symbionts in field-collected psyllid populations was determined: Sodalis was detected in 100% of field populations, while Spiroplasma was present in 82.5% of individuals. Phylogenetic analysis using 16S rDNA revealed that Sodalis infecting B. trigonica was more closely related to symbionts infecting weevils, stink bugs and tsetse flies than to those from psyllid species. Using fluorescent in situ hybridization and immunostaining, Sodalis was found to be localized inside the nuclei of the midgut cells and bacteriocytes. Spiroplasma was restricted to the cytoplasm of the midgut cells. We further show that a recently reported Bactericera trigonica densovirus (BtDNV), a densovirus infecting B. trigonica was detected in 100% of psyllids and has reduced titers inside CLso-infected psyllids by more than two-fold compared to CLso uninfected psyllids. The findings of this study will help to increase our understanding of psyllid–endosymbiont interactions.

Published

2020

7. Tsetse flies (Glossina morsitans morsitans) choose birthing sites guided by substrate cues with no evidence for a role of pheromones

Author

Andrea K. Adden, Lee R. Haines, Álvaro Acosta-Serrano, and Lucia L. Prieto-Godino

Subjects

General Immunology and Microbiology, Ecology,Evolution & Ethology, FOS: Clinical medicine, Neurosciences, General Medicine, General Agricultural and Biological Sciences, Genetics & Genomics, General Biochemistry, Genetics and Molecular Biology, General Environmental Science, Imaging, Developmental Biology

Abstract

Tsetse flies significantly impact public health and economic development in sub-Saharan African countries by transmitting the fatal disease African trypanosomiasis. Unusually, instead of laying eggs, tsetse birth a single larva that immediately burrows into the soil to pupate. Where the female chooses to larviposit is, therefore, crucial for offspring survival. Previous laboratory studies suggested that a putative larval pheromone, n -pentadecane, attracts gravid female Glossina morsitans morsitans to appropriate larviposition sites. However, this attraction could not be reproduced in field experiments. Here, we resolve this disparity by designing naturalistic laboratory experiments that closely mimic the physical characteristics found in the wild. We show that gravid G. m. morsitans were neither attracted to the putative pheromone nor, interestingly, to pupae placed in the soil. By contrast, females appear to choose larviposition sites based on environmental substrate cues. We conclude that, among the many cues that likely contribute to larviposition choice in nature, substrate features are a main determinant, while we failed to find evidence for a role of pheromones.

Published

2023

8. The Trypanosoma brucei MISP family of invariant proteins is co-expressed with BARP as triple helical bundle structures on the surface of salivary gland forms, but is dispensable for parasite development within the tsetse vector

Author

Aitor Casas-Sanchez, Raghavendran Ramaswamy, Samïrah Perally, Lee R. Haines, Clair Rose, Marcela Aguilera-Flores, Susana Portillo, Margot Verbeelen, Shahid Hussain, Laura Smithson, Cristina Yunta, Michael J. Lehane, Sue Vaughan, Jan van den Abbeele, Igor C. Almeida, Martin J. Boulanger, and Álvaro Acosta-Serrano

Subjects

Virology, Immunology, Genetics, Parasitology, Molecular Biology, Microbiology

Abstract

Trypanosoma brucei spp. develop into mammalian-infectious metacyclic trypomastigotes inside tsetse salivary glands. Besides acquiring a variant surface glycoprotein (VSG) coat, little is known about the metacyclic expression of invariant surface antigens. Proteomic analyses of saliva from T. brucei-infected tsetse flies identified, in addition to VSG and Brucei Alanine-Rich Protein (BARP) peptides, a family of glycosylphosphatidylinositol (GPI)-anchored surface proteins herein named as Metacyclic Invariant Surface Proteins (MISP) because of its predominant expression on the surface of metacyclic trypomastigotes. The MISP family is encoded by five paralog genes with >80% protein identity, which are exclusively expressed by salivary gland stages of the parasite and peak in metacyclic stage, as shown by confocal microscopy and immuno-high resolution scanning electron microscopy. Crystallographic analysis of a MISP isoform (MISP360) and a high confidence model of BARP revealed a triple helical bundle architecture commonly found in other trypanosome surface proteins. Molecular modelling combined with live fluorescent microscopy suggests that MISP N-termini are potentially extended above the metacyclic VSG coat, and thus could be tested as a transmission-blocking vaccine target. However, vaccination with recombinant MISP360 isoform did not protect mice against a T. brucei infectious tsetse bite. Lastly, both CRISPR-Cas9-driven knock out and RNAi knock down of all MISP paralogues suggest they are not essential for parasite development in the tsetse vector. We suggest MISP may be relevant during trypanosome transmission or establishment in the vertebrate’s skin.

Published

2023

9. Illuminating the Prevalence of Trypanosoma brucei s.l. in Glossina Using LAMP as a Tool for Xenomonitoring.

Author

Lucas J Cunningham, Jessica K Lingley, Lee R Haines, Joseph M Ndung'u, Stephen J Torr, and Emily R Adams

Subjects

Arctic medicine. Tropical medicine, RC955-962, Public aspects of medicine, RA1-1270

Abstract

BACKGROUND:As the reality of eliminating human African trypanosomiasis (HAT) by 2020 draws closer, the need to detect and identify the remaining areas of transmission increases. Here, we have explored the feasibility of using commercially available LAMP kits, designed to detect the Trypanozoon group of trypanosomes, as a xenomonitoring tool to screen tsetse flies for trypanosomes to be used in future epidemiological surveys. METHODS AND FINDINGS:The DNA extraction method was simplified and worked with the LAMP kits to detect a single positive fly when pooled with 19 negative flies, and the absolute lowest limit of detection that the kits were able to work at was the equivalent of 0.1 trypanosome per ml. The DNA from Trypanosoma brucei brucei could be detected six days after the fly had taken a blood meal containing dead trypanosomes, and when confronted with a range of non-target species, from both laboratory-reared flies and wild-caught flies, the kits showed no evidence of cross-reacting. CONCLUSION:We have shown that it is possible to use a simplified DNA extraction method in conjunction with the pooling of tsetse flies to decrease the time it would take to screen large numbers of flies for the presence of Trypanozoon trypanosomes. The use of commercially-available LAMP kits provides a reliable and highly sensitive tool for xenomonitoring and identifying potential sleeping sickness transmission sites.

Published

2016

10. Trypanosoma brucei colonizes the tsetse gut via an immature peritrophic matrix in the proventriculus

Author

Aitor Casas-Sanchez, Michael J. Lehane, Jaime Lisack, Alvaro Acosta-Serrano, Clair Rose, Markus Engstler, Carla Solórzano, Ian A. Prior, Marco Marcello, Alison J. Beckett, Ben Middlehurst, Lee R. Haines, and Naomi A. Dyer

Subjects

Microbiology (medical), Tsetse Flies, Trypanosoma brucei brucei, Immunology, Matrix (biology), Biology, Trypanosoma brucei, Applied Microbiology and Biotechnology, Microbiology, 03 medical and health sciences, wc_705, parasitic diseases, Genetics, medicine, Animals, Parasite hosting, qx_505, Peritrophic matrix, 030304 developmental biology, 0303 health sciences, qx_4, Salivary gland, 030306 microbiology, Proventriculus, Cell Biology, biology.organism_classification, medicine.disease, Animal trypanosomiasis, Gut Epithelium, medicine.anatomical_structure, qw_52

Abstract

The peritrophic matrix of blood-feeding insects is a chitinous structure that forms a protective barrier against oral pathogens and abrasive particles1. Tsetse flies transmit Trypanosoma brucei, which is the parasite that causes human sleeping sickness and is also partially responsible for animal trypanosomiasis in Sub-Saharan Africa. For this parasite to establish an infection in flies, it must first colonize the area between the peritrophic matrix and gut epithelium called the ectoperitrophic space. Although unproven, it is generally accepted that trypanosomes reach the ectoperitrophic space by penetrating the peritrophic matrix in the anterior midgut2,3,4. Here, we revisited this event using fluorescence- and electron-microscopy methodologies. We show that trypanosomes penetrate the ectoperitrophic space in which the newly made peritrophic matrix is synthesized by the proventriculus. Our model describes how these proventriculus-colonizing parasites can either migrate to the ectoperitrophic space or become trapped within peritrophic matrix layers to form cyst-like bodies that are passively pushed along the gut as the matrix gets remodelled. Furthermore, early proventricular colonization seems to be promoted by factors in trypanosome-infected blood that cause higher salivary gland infections and potentially increase parasite transmission.

Published

2020

11. Isolation in Natural Host Cell Lines of Wolbachia Strains wPip from the Mosquito Culex pipiens and wPap from the Sand Fly Phlebotomus papatasi

Author

James G. C. Hamilton, Lesley Bell-Sakyi, Laura Jones, Catherine Hartley, Alistair C. Darby, Benjamin L. Makepeace, Lee R. Haines, Alexandra Beliavskaia, and Lisa Luu

Subjects

Culex pipiens, Tetracycline, Science, media_common.quotation_subject, Lutzomyia longipalpis, Heterologous, mosquito, Insect, Tick, Phlebotomus papatasi, Article, tick cell line, Microbiology, parasitic diseases, medicine, Culicoides nubeculosus, qx_505, Wolbachia, media_common, qw_150, qx_4, biology, Host (biology), Intracellular parasite, fungi, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, qx_530, Insect Science, sand fly, medicine.drug

Abstract

Simple Summary Diverse strains of Wolbachia bacteria, carried by many arthropods, as well as some nematodes, interact in many different ways with their hosts. These include male killing, reproductive incompatibility, nutritional supplementation and suppression or enhancement of the transmission of diseases such as dengue and malaria. Consequently, Wolbachia have an important role to play in novel strategies to control human and livestock diseases and their vectors. Similarly, cell lines derived from insect hosts of Wolbachia constitute valuable research tools in this field. During the generation of novel cell lines from mosquito and sand fly vectors, we isolated two strains of Wolbachia and demonstrated their infectivity for cells from a range of other insects and ticks. These new insect cell lines and Wolbachia strains will aid in the fight against mosquitoes, sand flies and, potentially, ticks and the diseases that these arthropods transmit to humans and their domestic animals. Abstract Endosymbiotic intracellular bacteria of the genus Wolbachia are harboured by many species of invertebrates. They display a wide range of developmental, metabolic and nutritional interactions with their hosts and may impact the transmission of arboviruses and protozoan parasites. Wolbachia have occasionally been isolated during insect cell line generation. Here, we report the isolation of two strains of Wolbachia, wPip and wPap, during cell line generation from their respective hosts, the mosquito Culex pipiens and the sand fly Phlebotomus papatasi. wPip was pathogenic for both new C. pipiens cell lines, CPE/LULS50 and CLP/LULS56, requiring tetracycline treatment to rescue the lines. In contrast, wPap was tolerated by the P. papatasi cell line PPL/LULS49, although tetracycline treatment was applied to generate a Wolbachia-free subline. Both Wolbachia strains were infective for a panel of heterologous insect and tick cell lines, including two novel lines generated from the sand fly Lutzomyia longipalpis, LLE/LULS45 and LLL/LULS52. In all cases, wPip was more pathogenic for the host cells than wPap. These newly isolated Wolbachia strains, and the novel mosquito and sand fly cell lines reported here, will add to the resources available for research on host–endosymbiont relationships, as well as on C. pipiens, P. papatasi, L. longipalpis and the pathogens that they transmit.

Published

2021

12. Oxidative phosphorylation is required for powering motility and development of the sleeping sickness parasite Trypanosoma brucei within the tsetse fly vector

Author

Brice Rotureau, Alvaro Acosta-Serrano, Aitor Casas-Sanchez, Achim Schnaufer, Constentin Dieme, Caroline E. Dewar, Lee R. Haines, and Aline Crouzols

Subjects

ATP synthase, biology, fungi, Respiratory chain, Tsetse fly, Motility, Midgut, Oxidative phosphorylation, Trypanosoma brucei, biology.organism_classification, Cell biology, Kinetoplast, parasitic diseases, biology.protein

Abstract

The single-celled parasite Trypanosoma brucei causes sleeping sickness in humans and nagana in livestock and is transmitted by hematophagous tsetse flies. Lifecycle progression from mammalian bloodstream form to tsetse midgut form and, subsequently, infective salivary gland form depends on complex developmental steps and migration within different fly tissues. As the parasite colonises the glucose-poor insect midgut, its ATP production is thought to depend on activation of mitochondrial amino acid catabolism via oxidative phosphorylation. This process involves respiratory chain complexes and the F1FO-ATP synthase, and it requires protein subunits of these complexes that are encoded in the parasite’s mitochondrial DNA (kinetoplast or kDNA). Here we show that a progressive loss of kDNA-encoded functions correlates with an increasingly impaired ability of T. brucei to initiate and complete its development in the tsetse. First, parasites with a mutated F1FO-ATP synthase with a reduced capacity for oxidative phosphorylation can initiate differentiation from bloodstream to insect form, but they are unable to proliferate in vitro. Unexpectedly, these cells can still colonise the tsetse midgut. However, these parasites exhibit a motility defect and are severely impaired in colonising or migrating to subsequent tsetse tissues. Second, parasites with a fully disrupted F1FO-ATP synthase complex that is completely unable to produce ATP by oxidative phosphorylation can still differentiate to the first insect stage in vitro but die within a few days and cannot establish a midgut infection in vivo. Third, mutant parasites lacking kDNA entirely can initiate differentiation but die within 24 h. Together, these three scenarios show that efficient ATP production via oxidative phosphorylation is not essential for initial colonisation of the tsetse vector, but it is required to power trypanosome migration within the fly.

Published

2021

13. Wing length and host location in tsetse (Glossina spp.): implications for control using stationary baits

Author

Jennifer S. Lord, Cari van Schalkwyk, John W. Hargrove, Sinead English, James S. Patterson, Lee R. Haines, Stephen J. Torr, and G. A. Vale

Subjects

0301 basic medicine, Male, Veterinary medicine, Tsetse Flies, Tsetse Glossina, 030231 tropical medicine, Population, Flight, Animal/physiology, Tsetse Flies/anatomy & histology, Biology, Body size, Insect Control, lcsh:Infectious and parasitic diseases, Wings, Animal/anatomy & histology, 03 medical and health sciences, 0302 clinical medicine, Feeding behavior, Species Specificity, Mobile vehicle, Animals, Body Size, Wings, Animal, lcsh:RC109-216, education, education.field_of_study, Wing, Host (biology), Research, Age season annual effects, Insect Control/methods, Feeding Behavior, 030104 developmental biology, Infectious Diseases, Flight, Animal, Stationary and mobile baits, Wing length, Parasitology, Female, Eradication using targets, %22">Glossina

Abstract

Background It has been suggested that attempts to eradicate populations of tsetse (Glossina spp.) using stationary targets might fail because smaller, less mobile individuals are unlikely to be killed by the targets. If true, tsetse caught in stationary traps should be larger than those from mobile baits, which require less mobility on the part of the flies. Results Sampling tsetse in the Zambezi Valley of Zimbabwe, we found that the number of tsetse caught from stationary traps, as a percent of total numbers from traps plus a mobile vehicle, was ~5% for male G. morsitans morsitans (mean wing length 5.830 mm; 95% CI: 5.800–5.859 mm) and ~10% for females (6.334 mm; 95% CI: 6.329–6.338 mm); for G. pallidipes the figures were ~50% for males (6.830 mm; 95% CI: 6.821–6.838 mm) and ~75% for females (7.303 mm, 95% CI: 7.302–7.305 mm). As expected, flies of the smaller species (and the smaller sex) were less likely to be captured using stationary, rather than mobile sampling devices. For flies of a given sex and species the situation was more complex. Multivariable analysis showed that, for females of both species, wing lengths changed with ovarian age and the month, year and method of capture. For G. pallidipes, there were statistically significant interactions between ovarian age and capture month, year and method. For G. m. morsitans, there was only a significant interaction between ovarian age and capture month. The effect of capture method was, however, small in absolute terms: for G. pallidipes and G. m. morsitans flies caught on the mobile vehicle had wings only 0.24 and 0.48% shorter, respectively, than flies caught in stationary traps. In summary, wing length in field samples of tsetse varies with ovarian age, capture month and year and, weakly, with capture method. Suggestions that a target-based operation against G. f. fuscipes in Kenya caused a shift towards a smaller, less mobile population of tsetse, unavailable to the targets, failed to account for factors other than capture method. Conclusions The results are consistent with the successful use of targets to eradicate populations of tsetse in Zimbabwe. Until further, more nuanced, studies are conducted, it is premature to conclude that targets alone could not, similarly, be used to eradicate G. f. fuscipes populations in Kenya. Electronic supplementary material The online version of this article (10.1186/s13071-018-3274-x) contains supplementary material, which is available to authorized users.

Published

2019

14. Repurposing the orphan drug nitisinone to control the transmission of African trypanosomiasis

Author

Natalia Garcia Escude, Hanafy M. Ismail, Mark I. Paine, Mariana Silva dos Santos, Vincent O. Adung'a, Raquel J. Vionette-Amaral, Shannon Quek, James I. MacRae, Clair Rose, Simon C. Wagstaff, Lee R. Haines, Daniel K. Masiga, Aitor Casas-Sanchez, Laith Yakob, Pedro L. Oliveira, Seth M. Barribeau, Alvaro Acosta-Serrano, Marcos Sterkel, and Besansky, Nora J.

Subjects

Male, Biología, Enzyme Metabolism, Pharmacology, Biochemistry, Mice, Tyrosine aminotransferase, 0302 clinical medicine, Medical Conditions, wc_705, Biology (General), Amino Acids, Enzyme Chemistry, media_common, Mammals, 0303 health sciences, Organic Compounds, Gene silencing, Eukaryota, Neglected Diseases, Bees, 3. Good health, Blood, Physical Sciences, Metabolic Pathways, General Agricultural and Biological Sciences, Drug, Tsetse Flies, QH301-705.5, media_common.quotation_subject, Equines, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Hydroxyl Amino Acids, Humans, Horses, Rats, Wistar, Biology, Cyclohexanones, Organisms, Chemical Compounds, Drug Repositioning, Biology and Life Sciences, Proteins, Models, Theoretical, medicine.disease, Virology, Invertebrates, 030104 developmental biology, Trypanosomiasis, African, Nitrobenzoates, Nitisinone, Physiological Processes, Trypanosomiasis, 0301 basic medicine, Insecticides, Orphan Drug Production, Physiology, 4-Hydroxyphenylpyruvate Dioxygenase, Aromatic Amino Acids, RNA interference, Medicine and Health Sciences, African trypanosomiasis, qx_505, Tyrosine, Transmission (medicine), General Neuroscience, Ingestion, wc_695, Body Fluids, Insects, Chemistry, Infectious Diseases, Vertebrates, Metabolome, Female, Anatomy, medicine.drug, Research Article, wc_20, Arthropoda, Infectious Disease Control, 030231 tropical medicine, Orphan drug, Toxicity Tests, medicine, Animals, 030304 developmental biology, Infection Control, General Immunology and Microbiology, qu_4, Organic Chemistry, Rats, Metabolism, Amniotes, Enzymology, Rna interference, Zoology, Entomology

Abstract

Tsetse transmit African trypanosomiasis, which is a disease fatal to both humans and animals. A vaccine to protect against this disease does not exist so transmission control relies on eliminating tsetse populations. Although neurotoxic insecticides are the gold standard for insect control, they negatively impact the environment and reduce populations of insect pollinator species. Here we present a promising, environment-friendly alternative to current insecticides that targets the insect tyrosine metabolism pathway. A bloodmeal contains high levels of tyrosine, which is toxic to haematophagous insects if it is not degraded and eliminated. RNA interference (RNAi) of either the first two enzymes in the tyrosine degradation pathway (tyrosine aminotransferase (TAT) and 4-hydroxyphenylpyruvate dioxygenase (HPPD)) was lethal to tsetse. Furthermore, nitisinone (NTBC), an FDA-approved tyrosine catabolism inhibitor, killed tsetse regardless if the drug was orally or topically applied. However, oral administration of NTBC to bumblebees did not affect their survival. Using a novel mathematical model, we show that NTBC could reduce the transmission of African trypanosomiasis in sub-Saharan Africa, thus accelerating current disease elimination programmes., This study shows that tsetse flies, vectors of African trypanosomiasis, are highly susceptible to killing by nitisinone, a tyrosine catabolism inhibitor currently used to treat human metabolic diseases; this environment-friendly drug could facilitate elimination of African trypanosomiasis and other diseases transmitted by blood feeding insects.

Published

2021

15. Author response for 'Effects of maternal age and stress on offspring quality in a viviparous fly'

Author

Robert Leyland, Lee R. Haines, Sinead English, Antoine M G Barreaux, Michael B. Bonsall, Jennifer S. Lord, and Stephen J. Torr

Subjects

Offspring, media_common.quotation_subject, Stress (linguistics), Quality (business), Biology, Demography, media_common

Published

2020

16. Effects of maternal age and stress on offspring quality in a viviparous fly

Author

Robert Leyland, Antoine M G Barreaux, Stephen J. Torr, Sinead English, Michael B. Bonsall, Jennifer S. Lord, and Lee R. Haines

Subjects

Senescence, Aging, maternal allocation, senescence, tsetse, Offspring, media_common.quotation_subject, Population, Zoology, Physiology, Biology, Abortion, Intraspecific competition, Reproductive senescence, Pregnancy, qx_500, medicine, Humans, Reproductive history, qx_505, Mating, education, Ecology, Evolution, Behavior and Systematics, media_common, Starvation, education.field_of_study, Ecology, Reproduction, qx_650, Female, medicine.symptom, Maternal Age

Abstract

Many organisms show signs of deterioration with age in terms of survival and reproduction. We tested whether intraspecific variation in such senescence patterns can be driven by resource availability or reproductive history. We did this by manipulating nutritional stress and age at first reproduction and measuring age-dependent reproductive output in tsetse (Glossina morsitans morsitans), a viviparous fly with high maternal allocation. Across all treatments, offspring weight followed a bell-shaped curve with maternal age. Nutritionally stressed females had a higher probability of abortion and produced offspring with lower starvation tolerance. There was no evidence of an increased rate of reproductive senescence in nutritionally stressed females, or a reduced rate due to delayed mating, as measured by patterns of abortion, offspring weight or offspring starvation tolerance. Therefore, although we found evidence of reproductive senescence in tsetse, our results did not indicate that resource allocation trade-offs or costs of reproduction increase the rate of senescence.

Published

2020

17. An Intranuclear

Author

Saptarshi, Ghosh, Noa, Sela, Svetlana, Kontsedalov, Galina, Lebedev, Lee R, Haines, and Murad, Ghanim

Subjects

intranuclear bacteria, Sodalis, Spiroplasma, fungi, secondary endosymbiont, psyllid, Article, Candidatus Liberibacter solanacearum, Bactericera trigonica

Abstract

Endosymbionts harbored inside insects play critical roles in the biology of their insect host and can influence the transmission of pathogens by insect vectors. Bactericera trigonica infests umbelliferous plants and transmits the bacterial plant pathogen Candidatus Liberibacter solanacearum (CLso), causing carrot yellows disease. To characterize the bacterial diversity of B. trigonica, as a first step, we used PCR-restriction fragment length polymorphism (PCR-RFLP) and denaturing gradient gel electrophoresis (DGGE) analyses of 16S rDNA to identify Sodalis and Spiroplasma endosymbionts. The prevalence of both symbionts in field-collected psyllid populations was determined: Sodalis was detected in 100% of field populations, while Spiroplasma was present in 82.5% of individuals. Phylogenetic analysis using 16S rDNA revealed that Sodalis infecting B. trigonica was more closely related to symbionts infecting weevils, stink bugs and tsetse flies than to those from psyllid species. Using fluorescent in situ hybridization and immunostaining, Sodalis was found to be localized inside the nuclei of the midgut cells and bacteriocytes. Spiroplasma was restricted to the cytoplasm of the midgut cells. We further show that a recently reported Bactericera trigonica densovirus (BtDNV), a densovirus infecting B. trigonica was detected in 100% of psyllids and has reduced titers inside CLso-infected psyllids by more than two-fold compared to CLso uninfected psyllids. The findings of this study will help to increase our understanding of psyllid–endosymbiont interactions.

Published

2020

18. Killing of trypanosomatid parasites by a modified bovine host defense peptide, BMAP-18.

Author

Lee R Haines, Jamie M Thomas, Angela M Jackson, Brett A Eyford, Morteza Razavi, Cristalle N Watson, Brent Gowen, Robert E W Hancock, and Terry W Pearson

Subjects

Arctic medicine. Tropical medicine, RC955-962, Public aspects of medicine, RA1-1270

Abstract

BACKGROUND: Tropical diseases caused by parasites continue to cause socioeconomic devastation that reverberates worldwide. There is a growing need for new control measures for many of these diseases due to increasing drug resistance exhibited by the parasites and problems with drug toxicity. One new approach is to apply host defense peptides (HDP; formerly called antimicrobial peptides) to disease control, either to treat infected hosts, or to prevent disease transmission by interfering with parasites in their insect vectors. A potent anti-parasite effector is bovine myeloid antimicrobial peptide-27 (BMAP-27), a member of the cathelicidin family. Although BMAP-27 is a potent inhibitor of microbial growth, at higher concentrations it also exhibits cytotoxicity to mammalian cells. We tested the anti-parasite activity of BMAP-18, a truncated peptide that lacks the hydrophobic C-terminal sequence of the BMAP-27 parent molecule, an alteration that confers reduced toxicity to mammalian cells. METHODOLOGY/PRINCIPAL FINDINGS: BMAP-18 showed strong growth inhibitory activity against several species and life cycle stages of African trypanosomes, fish trypanosomes and Leishmania parasites in vitro. When compared to native BMAP-27, the truncated BMAP-18 peptide showed reduced cytotoxicity on a wide variety of mammalian and insect cells and on Sodalis glossindius, a bacterial symbiont of the tsetse vector. The fluorescent stain rhodamine 123 was used in immunofluorescence microscopy and flow cytometry experiments to show that BMAP-18 at low concentrations rapidly disrupted mitochondrial potential without obvious alteration of parasite plasma membranes, thus inducing death by apoptosis. Scanning electron microscopy revealed that higher concentrations of BMAP-18 induced membrane lesions in the parasites as early as 15 minutes after exposure, thus killing them by necrosis. In addition to direct killing of parasites, BMAP-18 was shown to inhibit LPS-induced secretion of tumour necrosis factor alpha (TNF-alpha), a cytokine that is associated with inflammation and cachexia (wasting) in sleeping sickness patients. As a prelude to in vivo applications, high affinity antibodies to BMAP-18 were produced in rabbits and used in immuno-mass spectrometry assays to detect the intact peptide in human blood and plasma. CONCLUSIONS/SIGNIFICANCE: BMAP-18, a truncated form of the potent antimicrobial BMAP-27, showed low toxicity to mammalian cells, insect cells and the tsetse bacterial symbiont Sodalis glossinidius while retaining an ability to kill a variety of species and life cycle stages of pathogenic kinetoplastid parasites in vitro. BMAP-18 also inhibited secretion of TNF-alpha, an inflammatory cytokine that plays a role in the cachexia associated with African sleeping sickness. These findings support the idea that BMAP-18 should be explored as a candidate for therapy of economically important trypanosome-infected hosts, such as cattle, fish and humans, and for paratransgenic expression in Sodalis glossinidius, a bacterial symbiont in the tsetse vector, as a strategy for interference with trypanosome transmission.

Published

2009

19. Cutaneous leishmaniasis and co-morbid major depressive disorder: A systematic review with burden estimates

Author

Waleed S. Al-Salem, Peter J. Hotez, Ahmed Alorfi, Julian Eaton, Freddie Bailey, Iván D. Vélez, Amina Olabi, Alvaro Acosta-Serrano, Karina Mondragon-Shem, Lee R. Haines, David H. Molyneux, Emily R. Adams, Jorge Alvar, and José Antonio Ruiz-Postigo

Subjects

0301 basic medicine, Comorbidity, Global Health, Global Burden of Disease, 0302 clinical medicine, Cost of Illness, Zoonoses, Prevalence, Medicine and Health Sciences, Psychology, Public and Occupational Health, Leishmaniasis, Depression (differential diagnoses), Depression, Incidence, Incidence (epidemiology), lcsh:Public aspects of medicine, Neglected Diseases, Socioeconomic Aspects of Health, Infectious Diseases, Major depressive disorder, Quality-Adjusted Life Years, Anatomy, Psychosocial, Research Article, Neglected Tropical Diseases, medicine.medical_specialty, lcsh:Arctic medicine. Tropical medicine, lcsh:RC955-962, 030231 tropical medicine, Leishmaniasis, Cutaneous, 03 medical and health sciences, Life Expectancy, Cutaneous leishmaniasis, Internal medicine, Mental Health and Psychiatry, Parasitic Diseases, medicine, Humans, Disease burden, Depressive Disorder, Major, Protozoan Infections, Mood Disorders, Public Health, Environmental and Occupational Health, Biology and Life Sciences, lcsh:RA1-1270, Tropical Diseases, medicine.disease, Quality-adjusted life year, Health Care, 030104 developmental biology, Face, Quality of Life, Head

Abstract

Background Major depressive disorder (MDD) associated with chronic neglected tropical diseases (NTDs) has been identified as a significant and overlooked contributor to overall disease burden. Cutaneous leishmaniasis (CL) is one of the most prevalent and stigmatising NTDs, with an incidence of around 1 million new cases of active CL infection annually. However, the characteristic residual scarring (inactive CL) following almost all cases of active CL has only recently been recognised as part of the CL disease spectrum due to its lasting psychosocial impact. Methods and findings We performed a multi-language systematic review of the psychosocial impact of active and inactive CL. We estimated inactive CL (iCL) prevalence for the first time using reported WHO active CL (aCL) incidence data that were adjusted for life expectancy and underreporting. We then quantified the disability (YLD) burden of co-morbid MDD in CL using MDD disability weights at three severity levels. Overall, we identified 29 studies of CL psychological impact from 5 WHO regions, representing 11 of the 50 highest burden countries for CL. We conservatively calculated the disability burden of co-morbid MDD in CL to be 1.9 million YLDs, which equalled the overall (DALY) disease burden (assuming no excess mortality in depressed CL patients). Thus, upon inclusion of co-morbid MDD alone in both active and inactive CL, the DALY burden was seven times higher than the latest 2016 Global Burden of Disease study estimates, which notably omitted both psychological impact and inactive CL. Conclusions Failure to include co-morbid MDD and the lasting sequelae of chronic NTDs, as exemplified by CL, leads to large underestimates of overall disease burden., Author summary Cutaneous leishmaniasis is a highly prevalent vector-borne disease affecting large parts of Latin America and the Middle East, as well as parts of Northern Africa. There are several types of Cutaneous leishmaniasis, almost all of which have an active phase characterized by a disfiguring lesion (typically on exposed parts of the body), which then becomes a permanent scar (the inactive phase). We recently published an article highlighting the impact of the inactive scarring phase of CL on affected individuals, which is associated with high levels of stigma. Nevertheless, this aspect of the disease is not considered in its own right when calculating the overall disease burden by the Global Burden of Disease (GBD) Studies. In this article we estimate the prevalence of depression (major depressive disorder) in cutaneous leishmaniasis, in both the active and inactive forms. We then show the contribution of inactive CL to the overall disease burden estimates when included, which is due to the large psychological impact it has on those affected by it. We also highlight the importance of further similar efforts for other NTDs which have a chronic course, and which are also not sufficiently included in disease burden calculations at present.

Published

2019

20. An Intranuclear Sodalis-Like Symbiont and Spiroplasma Coinfect the Carrot Psyllid, Bactericera trigonica (Hemiptera, Psylloidea)

Author

Murad Ghanim, Svetlana Kontsedalov, Lee R. Haines, Noa Sela, Saptarshi Ghosh, and Galina Lebedev

Subjects

Microbiology (medical), Sodalis, food.ingredient, intranuclear bacteria, media_common.quotation_subject, Spiroplasma, Insect, Microbiology, 03 medical and health sciences, food, Virology, Bactericera, qx_503, lcsh:QH301-705.5, 030304 developmental biology, media_common, 0303 health sciences, biology, 030306 microbiology, qw_138, fungi, secondary endosymbiont, Psylloidea, Midgut, biology.organism_classification, psyllid, Hemiptera, Candidatus Liberibacter solanacearum, qx_650, lcsh:Biology (General), Bactericera trigonica, Densovirus

Abstract

Endosymbionts harbored inside insects play critical roles in the biology of their insect host and can influence the transmission of pathogens by insect vectors. Bactericera trigonica infests umbelliferous plants and transmits the bacterial plant pathogen Candidatus Liberibacter solanacearum (CLso), causing carrot yellows disease. To characterize the bacterial diversity of B. trigonica, as a first step, we used PCR-restriction fragment length polymorphism (PCR-RFLP) and denaturing gradient gel electrophoresis (DGGE) analyses of 16S rDNA to identify Sodalis and Spiroplasma endosymbionts. The prevalence of both symbionts in field-collected psyllid populations was determined: Sodalis was detected in 100% of field populations, while Spiroplasma was present in 82.5% of individuals. Phylogenetic analysis using 16S rDNA revealed that Sodalis infecting B. trigonica was more closely related to symbionts infecting weevils, stink bugs and tsetse flies than to those from psyllid species. Using fluorescent in situ hybridization and immunostaining, Sodalis was found to be localized inside the nuclei of the midgut cells and bacteriocytes. Spiroplasma was restricted to the cytoplasm of the midgut cells. We further show that a recently reported Bactericera trigonica densovirus (BtDNV), a densovirus infecting B. trigonica was detected in 100% of psyllids and has reduced titers inside CLso-infected psyllids by more than two-fold compared to CLso uninfected psyllids. The findings of this study will help to increase our understanding of psyllid&ndash, endosymbiont interactions.

Published

2020

21. The crystal structure and localization of Trypanosoma brucei invariant surface glycoproteins suggest a more permissive VSG coat in the tsetse-transmitted metacyclic stage

Author

Alvaro Acosta-Serrano, Cristina Yunta, Raghavendran Ramaswamy, Michael J. Lehane, Marcela Aguilera-Flores, Samirah Perally, Lee R. Haines, Igor C. Almeida, Clair Rose, Martin J. Boulanger, and Aitor Casas-Sanchez

Subjects

chemistry.chemical_classification, 0303 health sciences, Coat, biology, 030231 tropical medicine, Cell, Trypanosoma brucei, biology.organism_classification, Epitope, Cell biology, 03 medical and health sciences, 0302 clinical medicine, medicine.anatomical_structure, Antigen, chemistry, Fluorescence microscope, medicine, Glycoprotein, Gene, 030304 developmental biology

Abstract

Trypanosoma bruceispp. develop into mammalian-infectious metacyclic trypomastigotes inside the tsetse salivary glands. Besides acquiring a variant surface glycoprotein (VSG) coat, nothing is known about expression of invariant surface antigens by the metacyclic stage. Proteomic analysis of saliva fromT. brucei-infected flies revealed a novel family of hypothetical GPI-anchored surface proteins herein named Metacyclic Invariant Surface Proteins (MISP). MISP are encoded by five homolog genes and share ~80% protein identity. The crystal structure of MISP N-terminus at 1.82 Å resolution revealed a triple helical bundle that shares key features with other trypanosome surface proteins. However, molecular modelling combined with live fluorescent microscopy suggest that MISP N-termini are extended above the metacyclic VSG coat, exposing immunogenic epitopes. Collectively, we suggest that the metacyclic cell surface architecture appears more permissive than bloodstream forms in terms of expression of invariant GPI-anchored glycoproteins, which could be exploited for the development of novel vaccines against African trypanosomiases.

Published

2018

22. Variant antigen repertoires in Trypanosoma congolense populations and experimental infections can be profiled from deep sequence data using universal protein motifs

Author

Mandy Sanders, Matthew Berriman, Aitor Casas-Sanchez, Moses Ogugo, Alvaro Acosta-Serrano, Lee R. Haines, Andrew P. Jackson, Harry Noyes, Kihara Absolomon, Sara Silva Pereira, and Steve Kemp

Subjects

0301 basic medicine, Male, Tsetse Flies, Trypanosoma congolense, 030231 tropical medicine, Population, Amino Acid Motifs, Method, Computational biology, Biology, Genome, Deep sequencing, 03 medical and health sciences, 0302 clinical medicine, parasitic diseases, Genetics, Antigenic variation, Animals, education, Gene, Genetics (clinical), education.field_of_study, Polymorphism, Genetic, Contig, Nucleic acid sequence, Sequence Analysis, DNA, biology.organism_classification, 030104 developmental biology, Trypanosoma, Variant Surface Glycoproteins, Trypanosoma

Abstract

African trypanosomes are vector-borne hemoparasites of humans and animals. In the mammal, parasites evade the immune response through antigenic variation. Periodic switching of the variant surface glycoprotein (VSG) coat covering their cell surface allows sequential expansion of serologically distinct parasite clones. Trypanosome genomes contain many hundreds of VSG genes, subject to rapid changes in nucleotide sequence, copy number, and chromosomal position. Thus, analyzing, or even quantifying, VSG diversity over space and time presents an enormous challenge to conventional techniques. Indeed, previous population genomic studies have overlooked this vital aspect of pathogen biology for lack of analytical tools. Here we present a method for analyzing population-scale VSG diversity in Trypanosoma congolense from deep sequencing data. Previously, we suggested that T. congolense VSGs segregate into defined “phylotypes” that do not recombine. In our data set comprising 41 T. congolense genome sequences from across Africa, these phylotypes are universal and exhaustive. Screening sequence contigs with diagnostic protein motifs accurately quantifies relative phylotype frequencies, providing a metric of VSG diversity, called the “variant antigen profile.” We applied our metric to VSG expression in the tsetse fly, showing that certain, rare VSG phylotypes may be preferentially expressed in infective, metacyclic-stage parasites. Hence, variant antigen profiling accurately and rapidly determines the T. congolense VSG gene and transcript repertoire from sequence data, without need for manual curation or highly contiguous sequences. It offers a tractable approach to measuring VSG diversity across strains and during infections, which is imperative to understanding the host–parasite interaction at population and individual scales.

Published

2018

23. Cutaneous Leishmaniasis and Conflict in Syria

Author

David M. Pigott, Louise A. Kelly-Hope, David H. Molyneux, Simon I. Hay, Krishanthi Subramaniam, Lee R. Haines, Alvaro Acosta-Serrano, and Waleed S. Al-Salem

Subjects

refugee camps, 0301 basic medicine, Microbiology (medical), Warfare, Veterinary medicine, Disease reservoir, Letter, Databases, Factual, Epidemiology, Expedited, Refugee, vector-borne infections, 030231 tropical medicine, Leishmaniasis, Cutaneous, lcsh:Medicine, parasites, lcsh:Infectious and parasitic diseases, 03 medical and health sciences, 0302 clinical medicine, Cutaneous leishmaniasis, medicine, Humans, lcsh:RC109-216, Leishmania major, Phlebotomus, Letters to the Editor, Socioeconomics, Leishmania, Geography, Syria, biology, Incidence, lcsh:R, fungi, Outbreak, social sciences, biology.organism_classification, medicine.disease, humanities, 030104 developmental biology, Infectious Diseases, Cutaneous Leishmaniasis and Conflict in Syria, Population Surveillance, Vector (epidemiology), sand fly

Abstract

To the Editor: War, infection, and disease have always made intimate bedfellows, with disease recrudescence characterizing most conflict zones (1). Recently, increasing violence from civil war and terrorist activity in the Middle East has caused the largest human displacement in decades. A neglected consequence of this tragedy has been the reemergence of a cutaneous leishmaniasis epidemic. Old World cutaneous leishmaniasis is one of the most prevalent insectborne diseases within the World Health Organization’s Eastern Mediterranean Region (2). Zoonotic cutaneous leishmaniasis is caused by the protozoan parasite Leishmania major, which is transmitted through the infectious bite of the female Phlebotomus papatasi sand fly; the animal reservoirs are the rodent genera Rhombomys, Psammomys, and Meriones. Anthroponotic cutaneous leishmaniasis is caused by L. tropica and transmitted between humans by the Ph. sergenti sand fly. Until 1960, cutaneous leishmaniasis prevalence in Syria was restricted to 2 areas to which it is endemic (Aleppo and Damascus); preconflict (c. 2010) incidence was 23,000 cases/year (3). However, in early 2013, an alarming increase to 41,000 cutaneous leishmaniasis cases was reported (3,4). The regions most affected are under Islamic State control; 6,500 cases occurred in Ar-Raqqah, Diyar Al-Zour, and Hasakah. Because these places are not historical hotspots of cutaneous leishmaniasis, this change might be attributed to the massive human displacement within Syria and the ecologic disruption of sand fly (Ph. papatasi) habitats. According to the United Nations High Commissioner for Refugees, >4.2 million Syrians have been displaced into neighboring countries; Turkey, Lebanon, and Jordan have accepted most of these refugees. As a result, cutaneous leishmaniasis has begun to emerge in areas where displaced Syrians and disease reservoirs coexist (5). According to the Lebanese Ministry of Health, during 2000–2012, only 6 cutaneous leishmaniasis cases were reported in Lebanon. However in 2013 alone, 1,033 new cases were reported, of which 96.6% occurred among the displaced Syrian refugee populations (5). Similarly in Turkey, nonendemic parasite strains L. major and L. donovani were introduced by incoming refugees (6). Many of the temporary refugee settlements are predisposed to increased risk because of malnutrition, poor housing, absence of clean water, and inadequate sanitation. The combination of favorable climate, abundant sand fly populations, displaced refugees, and deficient medical facilities and services has created an environment conducive to cutaneous leishmaniasis reemergence. For example, refugee settlements in Nizip in southern Turkey have reported several hundred cases (7). Using current datasets published in English and Arabic, we mapped cutaneous leishmaniasis prevalence within Syria and its neighboring countries (Figure). Our results demonstrate that cutaneous leishmaniasis prevalence coincides with the presence of refugee camps (Figure, panel A), which is plausible given the strong association between disease outbreaks and refugee settlements (8). The deterioration of Syrian health systems, including the cessation of countrywide vector control programs, has created an ideal environment for disease outbreaks (9). Likewise, the sand fly vectors are widely distributed throughout the Middle East; expansive Ph. papatasi and Ph. sergenti sand fly populations exist in Syria and Iraq (4). The presence of these vectors in regions of instability can create new cutaneous leishmaniasis foci, which might have debilitating, and often stigmatizing, consequences for residents and deployed military personnel (10). In addition, the distribution of Leishmania spp. overlaps with sand fly habitats (Figure, panel B) and disease reservoirs (W. Al-Salem, unpub. data). Consequently, the movement of large refugee populations into regions that are ill-equipped to manage imported cutaneous leishmaniasis has resulted in outbreaks in Turkey and Lebanon (5,6). Figure Cutaneous leishmaniasis prevalence within Syria and neighboring countries of the World Health Organization’s Eastern Mediterranean Region, 2013. A) Prevalence among refugee camps. Case data were taken from http://datadryad.org/resource/doi:10.5061/dryad.05f5h ... Our findings emphasize the importance of contemporaneous disease tracking to identify human populations at highest disease risk. To ameliorate the current cutaneous leishmaniasis crisis, particularly during the winter when cases start to appear, accurate disease monitoring and strategic training of persons based within refugee camps (medical staff, aid workers, volunteers, and military personnel) needs to be prioritized. Moreover, clinicians and other medical personnel residing in refugee-hosting countries must be suitably trained to diagnose cutaneous leishmaniasis because other local diseases (e.g., sarcoidosis and cutaneous tuberculosis) can have similar manifestations. Along with vector and rodent control, new cutaneous leishmaniasis outbreaks should be managed by prompt diagnosis and treatment, which are even more pertinent given that L. tropica–associated cutaneous leishmaniasis typically is resistant to several treatment regimens. In summary, the coexistence of sand fly populations and Leishmania spp. within refugee camps, together with the considerable influx of persons who already have cutaneous leishmaniasis, create a dangerous cocktail that can lead to an outbreak unprecedented in modern times.

Published

2016

24. Understanding the transmission dynamics of Leishmania donovani to provide robust evidence for interventions to eliminate visceral leishmaniasis in Bihar, India

Author

Richard M. Poché, David Weetman, Shyam Sundar, Michael A. Miles, Sarah Jervis, Margriet den Boer, Caryn Bern, Mark J. I. Paine, Simon L. Croft, Albert Picado, Erin Dilger, Angela F Harris, Pradeep Das, Graham F. Medley, Paul D. Ready, Rajesh Garlapati, Mark Rowland, Janet Hemingway, Sake J. de Vlas, Lee R. Haines, Alvaro Acosta-Serrano, Alexandra Chaskopoulou, Marleen Boelaert, Mary M. Cameron, Sakib Burza, Matthew E. Rogers, Geraldine M. Foster, Michael Coleman, T. Déirdre Hollingsworth, Lloyd A. C. Chapman, Orin Courtenay, and Public Health

Subjects

0301 basic medicine, Veterinary medicine, Cluster-randomized-trail, Indoor residual spraying, Mycology & Parasitology, Review, law.invention, 0302 clinical medicine, law, Phlebotomus, Indian sub-continent, Lasting insecticidal nets, Visceral leishmaniasis, Bangladesh, Disease Eradication, biology, Risk-factors, Phlebotomine sand flies, Transmission (mechanics), Infectious Diseases, Medical Microbiology, Leishmaniasis, Visceral, Life Sciences & Biomedicine, Argentipes, Elimination, 030231 tropical medicine, India, Context (language use), Public Health And Health Services, 03 medical and health sciences, Kala-Azar, Nepal, SDG 3 - Good Health and Well-being, Environmental health, Control, medicine, Animals, Humans, Transmission, Subcontinent, Science & Technology, Leishmaniasis, medicine.disease, biology.organism_classification, Vector control, 030104 developmental biology, Vector (epidemiology), Phlebotomus argentipes, Parasitology, RA, Leishmania donovani

Abstract

Visceral Leishmaniasis (VL) is a neglected vector-borne disease. In India, it is transmitted to humans by Leishmania donovani-infected Phlebotomus argentipes sand flies. In 2005, VL was targeted for elimination by the governments of India, Nepal and Bangladesh by 2015. The elimination strategy consists of rapid case detection, treatment of VL cases and vector control using indoor residual spraying (IRS). However, to achieve sustained elimination of VL, an appropriate post elimination surveillance programme should be designed, and crucial knowledge gaps in vector bionomics, human infection and transmission need to be addressed. This review examines the outstanding knowledge gaps, specifically in the context of Bihar State, India.\ud \ud The knowledge gaps in vector bionomics that will be of immediate benefit to current control operations include better estimates of human biting rates and natural infection rates of P. argentipes, with L. donovani, and how these vary spatially, temporally and in response to IRS. The relative importance of indoor and outdoor transmission, and how P. argentipes disperse, are also unknown. With respect to human transmission it is important to use a range of diagnostic tools to distinguish individuals in endemic communities into those who: 1) are to going to progress to clinical VL, 2) are immune/refractory to infection and 3) have had past exposure to sand flies.\ud \ud It is crucial to keep in mind that close to elimination, and post-elimination, VL cases will become infrequent, so it is vital to define what the surveillance programme should target and how it should be designed to prevent resurgence. Therefore, a better understanding of the transmission dynamics of VL, in particular of how rates of infection in humans and sand flies vary as functions of each other, is required to guide VL elimination efforts and ensure sustained elimination in the Indian subcontinent. By collecting contemporary entomological and human data in the same geographical locations, more precise epidemiological models can be produced. The suite of data collected can also be used to inform the national programme if supplementary vector control tools, in addition to IRS, are required to address the issues of people sleeping outside.

Published

2016

25. Prolonged gene knockdown in the tsetse flyGlossinaby feeding double stranded RNA

Author

Michael J. Lehane, Lee R. Haines, Deirdre Walshe, and Stella Lehane

Subjects

Trypanosoma, Gene knockdown, Tsetse Flies, biology, fungi, Tsetse fly, RNA, biology.organism_classification, Molecular biology, RNA silencing, Gene Expression Regulation, RNA interference, Gene Knockdown Techniques, Insect Science, parasitic diseases, Gene expression, Genetics, Animals, Gene Silencing, Molecular Biology, Gene, RNA, Double-Stranded

Abstract

Reverse genetic studies based on RNA interference (RNAi) have revolutionized analysis of gene function in most insects. However the necessity of injecting double stranded RNA (dsRNA) inevitably compromises many investigations particularly those on immunity. Additionally, injection of tsetse flies often causes significant mortality. We demonstrate, at transcript and protein level, that delivering dsRNA in the bloodmeal to Glossina morsitans morsitans is as effective as injection in knockdown of the immunoresponsive midgut-expressed gene TsetseEP. However, feeding dsRNA fails to knockdown the fat body expressed transferrin gene, 2A192, previously shown to be silenced by dsRNA injection. Mortality rates of the dsRNA fed flies were significantly reduced compared to injected flies 14 days after treatment (Fed: 10.1%+/- 1.8%; injected: 37.9% +/- 3.6% (Mean +/- SEM)). This is the first demonstration in Diptera of gene knockdown by feeding and the first example of knockdown in a blood-sucking insect by including dsRNA in the bloodmeal.

Published

2009

26. Increased expression of unusual EP repeat-containing proteins in the midgut of the tsetse fly (Glossina) after bacterial challenge

Author

Michael J. Lehane, Lee R. Haines, Angela M. Jackson, J D Haddow, Jamie M. Thomas, Ayako Yamaguchi, and Terry W. Pearson

Subjects

Immunogen, Tsetse Flies, Amino Acid Motifs, Molecular Sequence Data, Biochemistry, Epitope, Epitopes, parasitic diseases, Hemolymph, Animals, Amino Acid Sequence, Molecular Biology, Peptide sequence, biology, fungi, Sodalis glossinidius, Tsetse fly, Midgut, Proventriculus, Bacterial Infections, biology.organism_classification, Molecular biology, Insect Science, Insect Proteins, Digestive System

Abstract

Proteins containing a glutamic acid-proline (EP) repeat epitope were immunologically detected in midguts from eight species of Glossina (tsetse flies). The molecular masses of the tsetse EP proteins differed among species groups. The amino acid sequence of one of these proteins, from Glossina palpalis palpalis, was determined and compared to the sequence of a homologue, the tsetse midgut EP protein of Glossina in. morsitans. The extended EP repeat domains comprised between 36% (G. in. morsitans) and 46% (G. p. palpalis) of the amino acid residues, but otherwise the two polypeptide chains shared most of their sequences and predicted functional domains. The levels of expression of tsetse EP protein in adult teneral midguts were markedly higher than in midguts from larvae. The EP protein was detected by immunoblotting in the fat body, proventriculus and midgut, the known major immune tissues of tsetse and is likely secreted as it was also detected in hemolymph. The EP protein was not produced by the bacterial symbionts of tsetse midguts as determined by genome analysis of Wigglesmorthia glossinidia and immunoblot analysis of Sodalis glossinidius. Bacterial challenge of G. m. morsitans, by injection of live E. coli, induced augmented expression of the tsetse EP protein. The presence of EP proteins in a wide variety of tsetse, their constitutive expression in adult fat body and midguts and their upregulation after immunogen challenge suggest they play an important role as a component of the immune system in tsetse. (c) 2005 Elsevier Ltd. All rights reserved.

Published

2005

27. Inhibition of PACAP Activity by a Receptor Antagonist Results in Changes in Cell Cycle and Apoptotic Proteins in Chick Neuroblasts

Author

Terry W. Pearson, Lee R. Haines, Nancy M. Sherwood, and Nola M. Erhardt

Subjects

medicine.drug_class, Receptors, Pituitary Adenylate Cyclase-Activating Polypeptide, Ribosome biogenesis, Apoptosis, Receptors, Cell Surface, Endogeny, Chick Embryo, Biology, Mitochondrial Proteins, Cellular and Molecular Neuroscience, Neuroblast, medicine, Animals, Nerve Growth Factors, Cycloheximide, Enzyme Inhibitors, Receptor, Cells, Cultured, Neurons, Protein Synthesis Inhibitors, Neurotransmitter Agents, Tumor Suppressor Proteins, Cell Cycle, Neuropeptides, Cell Differentiation, General Medicine, Cell cycle, Staurosporine, Receptor antagonist, Molecular biology, Cell biology, Isotope Labeling, Pituitary Adenylate Cyclase-Activating Polypeptide, Apoptosome

Abstract

We showed previously that early chick neuroblasts stop proliferating and undergo apoptosis when deprived of endogenous pituitary adenylate cyclase-activating polypeptide (PACAP). To identify proteins involved in these processes, we blocked the primary PACAP receptor and determined protein changes using isotope-coded affinity tag (ICAT) analysis. Cell cycle exit was characterized by a decrease in proteins regulating ribosome biogenesis and protein translation. Apoptosis was linked directly to a tumor suppressor that increases apoptosome activity and indirectly to reduced mitochondrial activity. ICAT analysis, combined with flow cytometric analysis, suggested that some cells were differentiating, rather than undergoing apoptosis. In summary, we have confirmed that withdrawal of PACAP from early chick neuroblasts causes cell cycle exit and apoptosis, and identified proteins involved in proliferation, exit, apoptosis, and possibly differentiation.

Published

2005

28. Mass Spectrometric Quantitation of Peptides and Proteins Using Stable Isotope Standards and Capture by Anti-Peptide Antibodies (SISCAPA)

Author

Darryl B. Hardie, Terry W. Pearson, Robert W. Olafson, N. Leigh Anderson, Lee R. Haines, and Norman G. Anderson

Subjects

Mass spectrometric immunoassay, Spectrometry, Mass, Electrospray Ionization, Time Factors, alpha 1-Antichymotrypsin, In silico, Peptide, Biochemistry, Chromatography, Affinity, Mass Spectrometry, Antigen, Hemopexin, Humans, Nanotechnology, Ions, chemistry.chemical_classification, Chromatography, biology, Interleukin-6, Tumor Necrosis Factor-alpha, Chemistry, Elution, Proteins, Blood Proteins, General Chemistry, Antibodies, Anti-Idiotypic, Protein Structure, Tertiary, Polyclonal antibodies, biology.protein, Antibody, Peptides, Haptens, Chromatography, Liquid

Abstract

A method (denoted SISCAPA) for quantitation of peptides in complex digests is described. In the method, anti-peptide antibodies immobilized on 100 nanoliter nanoaffinity columns are used to enrich specific peptides along with spiked stable-isotope-labeled internal standards of the same sequence. Upon elution from the anti-peptide antibody supports, electrospray mass spectrometry is used to quantitate the peptides (natural and labeled). In a series of pilot experiments, tryptic test peptides were chosen for four proteins of human plasma (hemopexin, alpha1 antichymotrypsin, interleukin-6, and tumor necrosis factor-alpha) from a pool of 10,203 in silico tryptic peptide candidates representing 237 known plasma components. Rabbit polyclonal antibodies raised against the chosen peptide sequences were affinity purified and covalently immobilized on POROS supports. Binding and elution from these supports was shown to provide an average 120-fold enrichment of the antigen peptide relative to others, as measured by selected ion monitoring (SIM) or selected reaction monitoring (SRM) electrospray mass spectrometry. The columns could be recycled with little loss in binding capacity, and generated peptide ion current measurements with cycle-to-cycle coefficients of variation near 5%. Anti-peptide antibody enrichment will contribute to increased sensitivity of MS-based assays, particularly for lower abundance proteins in plasma, and may ultimately allow substitution of a rapid bind/elute process for the time-consuming reverse phase separation now used as a prelude to online MS peptide assays. The method appears suitable for rapid generation of assays for defined proteins, and should find application in the validation of diagnostic protein panels in large sample sets.

Published

2004

29. An Effective and Rapid Method for Functional Characterization of Immunoadsorbents Using POROS Beads and Flow Cytometry

Author

Terry W. Pearson, Anderson Nl, and Lee R. Haines

Subjects

Analyte, Chromatography, medicine.diagnostic_test, biology, Chemistry, medicine.drug_class, Peptide binding, General Chemistry, Immunosorbents, Monoclonal antibody, Biochemistry, Flow cytometry, Antigen, medicine, biology.protein, Protein G, Alexa Fluor

Abstract

To facilitate the construction, functional characterization, and use of immunoadsorbents, we have developed a flow cytometry method that allows rapid assessment of large numbers of particle-bound antibodies. Protein G derivitized POROS beads were used to bind affinity-purified antibodies specific for synthetic peptides designed from human plasma proteins. The antibodies were covalently coupled to the beads and used to capture and release synthetic peptides that had been labeled at the C-terminus with the fluorochrome Alexa Fluor 488. Antibody coupling and specificity of antigen binding and release were measured by analysis of the POROS affinity beads by flow cytometry. The affinity-capture matrixes were also used through several antigen-binding and release cycles without loss of peptide binding efficiency. The ability to produce and characterize extremely small amounts of POROS affinity matrices will facilitate their use in protein microchemical procedures such as protein chip technology, monoclonal antibody screening and mass spectrometry, applications where analytes are limiting or present in low abundance in complex mixtures.

Published

2004

30. Genome sequence of the tsetse fly (Glossina morsitans): vector of African trypanosomiasis

Author

George F. Obiero, Victor Chukwudi Osamor, Atsushi Toyoda, Apollo Simon Peter Balyeidhusa, Cheolho Sim, Paul O. Mireji, Jelle Caers, Serap Aksoy, Irene Omedo, Jan Van Den Abbeele, Lucien Manga, Wanqi Hu, Daniel Lawson, Tadashi Imanishi, Sing-Hoi Sze, Jeffery W. Jones, Sumir Panji, Erich Loza Telleria, Mandy Sanders, Joy J. Winzerling, Dawn L. Geiser, Atway R. Msangi, Joshua B. Benoit, Sandy J. Macdonald, Junichi Watanabe, James Cotton, Francesca Scolari, Steven G. Nyanjom, Linda M. Field, George Githinji, Vineet K. Sharma, José M. C. Ribeiro, Furaha Mramba, Stella Lehane, Shuhua Fu, Marco Falchetto, Imna I. Malele, Michael A. Riehle, Tulika P. Srivastava, Hugh M. Robertson, Immo A. Hansen, Mmule Makgamathe, Caleb K. Kibet, Philippe Solano, Alan Christoffels, Yoshihiro Kawahara, Megan E. Meuti, Nicola Mulder, Patrick Wincker, Gerd Gäde, Zahra Jalali Sefid Dashti, Heather G. Marco, Sheila C. Ommeh, Veronika Michalkova, Cher-Pheng Ooi, Geoffrey M. Attardo, Oliver Manangwa, David L. Denlinger, Alistair C. Darby, Todd D. Taylor, Daniel S.T. Hughes, Mark Wamalwa, Michael W. Gaunt, Daphne Q.-D. Pham, Rosaline W. Macharia, Chinyere K. Okoro, Lee R. Haines, Masahira Hattori, Markus Friedrich, Jingwen Wang, Aaron A. Baumann, Jing-Jiang Zhou, Martin Aslett, Judith H. Willis, Deirdre Walshe, Justin T. Peyton, Alvaro Acosta-Serrano, Loyce M. Okedi, Ludvik M. Gomulski, Johnson Kinyua, Daniel K. Masiga, Mathurin Koffi, J.J.O. Koekemoer, Corey L. Brelsfoard, Gordon William Harkins, Geoffrey H. Siwo, Guy Caljon, Michael A. Quail, Grace Murilla, Anna K. Snyder, Adele Kruger, Gavin H. Thomas, Anna R. Malacrida, Patrick P. Abila, Liliane Schoofs, Rosemary Bateta, Martin T. Swain, Michael J. Lehane, Richard Gregory, Kostas Bourtzis, Brian L. Weiss, Eleanor J Stanley, Zhijian Tu, Matthew Berriman, Winston Hide, David P. Price, Yutaka Suzuki, Maxwell J. Scott, Aaron M. Tarone, Joanna E. Auma, Johnson O. Ouma, Christiane Hertz-Fowler, Alia Benkahla, Karyn Megy, Sophie Ravel, Noboru Inoue, Feziwe Mpondo, Sarah Mwangi, Yeya T. Touré, Florence N. Wamwiri, Clair Rose, Neil D. Rawlings, George Tsiamis, Thiago Luiz, Peter Arensburger, Mario Jonas, Wesley C. Warren, Rita V. M. Rio, Richard K. Wilson, Heikki Lehväslaiho, Denis M. Larkin, Urvashi N. Ramphul, Qirui Zhang, Dawn Stephens, Neil Hall, Kevin K. Marucha, Ryuichi Sakate, Institut de Recherche pour le Développement (IRD [France-Sud]), Genoscope - Centre national de séquençage [Evry] (GENOSCOPE), Université Paris-Saclay-Direction de Recherche Fondamentale (CEA) (DRF (CEA)), Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Commissariat à l'énergie atomique et aux énergies alternatives (CEA), Laboratoire de Parasitologie Médicale, Biotechnologies et Biomolécules (LR11IPT06), Institut Pasteur de Tunis, and Réseau International des Instituts Pasteur (RIIP)-Réseau International des Instituts Pasteur (RIIP)

Subjects

MESH: Sequence Analysis, DNA, MESH: Insect Vectors/physiology, Genome, Insect, MESH: Insect Vectors/genetics, Genes, Insect, MESH: Genes, Insect, Genome, MESH: Insect Vectors/microbiology, Salivary Glands, MESH: Genome, Insect, 0302 clinical medicine, African trypanosomiasis, MESH: Animals, Genetics, MESH: Salivary Glands/physiology, 0303 health sciences, Multidisciplinary, MESH: Symbiosis, biology, Microbiota, Reproduction, MESH: Tsetse Flies/genetics, MESH: Tsetse Flies/parasitology, [SDV.MP]Life Sciences [q-bio]/Microbiology and Parasitology, Blood, MESH: Feeding Behavior, MESH: Insect Proteins/physiology, Insect Proteins, Wolbachia, MESH: Trypanosoma/physiology, Female, Trypanosoma, Tsetse Flies, MESH: Tsetse Flies/microbiology, MESH: Trypanosomiasis, African/transmission, 030231 tropical medicine, Molecular Sequence Data, Sensation, MESH: Wolbachia/physiology, MESH: Molecular Sequence Annotation, Article, MESH: Sensation/genetics, 03 medical and health sciences, medicine, MESH: Blood, MESH: Microbiota, Animals, MESH: Reproduction/genetics, Symbiosis, Gene, 030304 developmental biology, Whole genome sequencing, MESH: Insect Vectors/parasitology, MESH: Molecular Sequence Data, MESH: Insect Proteins/genetics, MESH: Salivary Glands/parasitology, Tsetse fly, Molecular Sequence Annotation, Feeding Behavior, Sequence Analysis, DNA, biology.organism_classification, medicine.disease, Insect Vectors, Trypanosomiasis, African, Vector (epidemiology), MESH: Tsetse Flies/physiology, MESH: Wolbachia/genetics, Trypanosomiasis, MESH: Female

Abstract

Africa's Bane Tsetse are blood-feeding, fast-flying flies that transmit a range of Trypanosoma spp. protozoan pathogens, which cause sleeping sickness in humans and their nagana in their livestock. The International Glossina Genome Initiative (p. 380 ) sequenced the genome of Glossina morsitans and identified the genes for many attributes of the tsetse's remarkable biology, including viviparity and the expression of analogs of mammalian milk proteins. Tsetse are host to several specific symbionts that appear to synthesize essential nutrients for the fly and also to hitherto undiscovered parasitoid-derived viruses. Deeper exploration of this genome will reveal what makes these fly species so host- and trypanosome specific.

Published

2014

31. An investigation into the protein composition of the teneral Glossina morsitans morsitans peritrophic matrix

Author

Clair Rose, Rodrigo Belmonte, Stuart D Armstrong, Gemma Molyneux, Lee R Haines, Michael J Lehane, Jonathan Wastling, and Alvaro Acosta-Serrano

Subjects

Male, Trypanosoma, lcsh:Arctic medicine. Tropical medicine, Glossina, Arthropoda, Proteome, Tsetse Flies, lcsh:RC955-962, Tsetse Fly, Epidemiology, Pathogenesis, Protozoology, Disease Vectors, Pathology and Laboratory Medicine, Microbiology, Vector Biology, Mass Spectrometry, Tandem Mass Spectrometry, Medicine and Health Sciences, Animals, Protozoans, lcsh:Public aspects of medicine, QH, Organisms, Biology and Life Sciences, Proteins, lcsh:RA1-1270, Invertebrates, Parasitic Protozoans, Insects, Gastrointestinal Tract, Host-Pathogen Interactions, Parasitology, Research Article, Chromatography, Liquid

Abstract

Background Tsetse flies serve as biological vectors for several species of African trypanosomes. In order to survive, proliferate and establish a midgut infection, trypanosomes must cross the tsetse fly peritrophic matrix (PM), which is an acellular gut lining surrounding the blood meal. Crossing of this multi-layered structure occurs at least twice during parasite migration and development, but the mechanism of how trypanosomes do so is not understood. In order to better comprehend the molecular events surrounding trypanosome penetration of the tsetse PM, a mass spectrometry-based approach was applied to investigate the PM protein composition using Glossina morsitans morsitans as a model organism. Methods PMs from male teneral (young, unfed) flies were dissected, solubilised in urea/SDS buffer and the proteins precipitated with cold acetone/TCA. The PM proteins were either subjected to an in-solution tryptic digestion or fractionated on 1D SDS-PAGE, and the resulting bands digested using trypsin. The tryptic fragments from both preparations were purified and analysed by LC-MS/MS. Results Overall, nearly 300 proteins were identified from both analyses, several of those containing signature Chitin Binding Domains (CBD), including novel peritrophins and peritrophin-like glycoproteins, which are essential in maintaining PM architecture and may act as trypanosome adhesins. Furthermore, 27 proteins from the tsetse secondary endosymbiont, Sodalis glossinidius, were also identified, suggesting this bacterium is probably in close association with the tsetse PM. Conclusion To our knowledge this is the first report on the protein composition of teneral G. m. morsitans, an important vector of African trypanosomes. Further functional analyses of these proteins will lead to a better understanding of the tsetse physiology and may help identify potential molecular targets to block trypanosome development within the tsetse., Author Summary African trypanosomes are transmitted by the haematophagous tsetse vector. For transmission to occur, bloodmeal ingested trypanosomes must overcome numerous barriers imposed by the fly. The first obstacle is the crossing of peritrophic matrix (PM), a cell-free structure that protects the midgut epithelial cells from coming under attack by the hosts' digestive enzymes, aids in water retention and helps prevent harmful pathogens from establishing a systemic infection. Trypanosomes cross the tsetse PM at least twice in their development but how they do so remains to be elucidated. Despite being a recognised barrier to trypanosome infections, there is limited knowledge of the molecular components of the tsetse PM. In this study we identified nearly 300 PM proteins using two mass spectrometry approaches. Several of the identified components were peritrophins, which are a key group of glycoproteins essential for PM integrity. In addition, we detected proteins from Sodalis glossinidius, a commensal bacterium linked to increased susceptibility to trypanosome infection in tsetse. Our study provides the first comprehensive identification of proteins from the tsetse PM, which provides a starting point for research into potential targets for vector control.

Published

2014

32. Analysis of Kudoa thyrsites (Myxozoa: Myxosporea) spore antigens using monoclonal antibodies

Author

M L Ken, J C Chase, Terry W. Pearson, Robert W. Olafson, D. J. Whitaker, Morag Stewart, J A Dawson-Coates, Lee R. Haines, and J D Haddow

Subjects

Spores, medicine.drug_class, Immunoblotting, Salmo salar, Antigens, Protozoan, Aquatic Science, Monoclonal antibody, Immunofluorescence, Epitope, Myxosporea, Microbiology, Fish Diseases, Mice, Species Specificity, medicine, Animals, Muscle, Skeletal, Kudoa thyrsites, Protozoan Infections, Animal, Ecology, Evolution, Behavior and Systematics, Mice, Inbred BALB C, Hybridomas, Myxozoa, biology, medicine.diagnostic_test, fungi, Antibodies, Monoclonal, Eukaryota, Flow Cytometry, biology.organism_classification, Spore, Molecular Weight, Microscopy, Fluorescence, Kudoa

Abstract

A method employing Percoll gradient centrifugation was developed to purify Kudoa thyrsites spores from somatic muscle tissue of Atlantic salmon Salmo salar. Highly purified spores were then used to immunize inbred BALB/c mice for derivation of hybridomas secreting Kudoa-specific monoclonal antibodies (mAbs). Analysis of mAbs by immunofluorescence microscopy and flow cytometry showed that several were specific for antigens on the surface of K. thyrsites spores whereas other mAbs reacted with polar capsules or with polar filaments of spores of K. thyrsites, K. paniformis and K. crumena. Immunoblots on spore lysates using the surface-binding mAbs showed a broad band of 46 to > 220 kDa, whereas mAbs specific for antigens of polar capsules and polar filaments detected sharper bands of various molecular masses, depending on the Kudoa species. The dominant epitope of the K. thyrsites spore surface antigen was shown to be carbohydrate as determined by its sensitivity to treatment with anhydrous trifluoromethane sulfonic acid and by its resistance to treatment with Proteinase K. Immunofluorescence microscopy using the K. thyrsites-specific mAbs on isolated, intact, permeabilized plasmodia and on thin sections of somatic muscle tissue containing plasmodia revealed intense labeling of spores both within the spore-producing plasmodia and in the flesh of infected Atlantic salmon. As few as 100 spores were detected by immunoblotting, indicating that these mAbs have potential for use in developing a field-based diagnostic test.

Published

2001

33. Examining the tsetse teneral phenomenon and permissiveness to trypanosome infection

Author

Lee R. Haines

Subjects

Microbiology (medical), Permissiveness, Trypanosoma, Glossina, Tsetse Flies, Immunology, Zoology, Biology, Microbiology, teneral phenomenon, Host-Parasite Interactions, Mini Review Article, Immunity, medicine, Parasite hosting, Animals, African trypanosomiasis, Peritrophic matrix, vector competence, fungi, Midgut, tsetse symbionts, medicine.disease, biology.organism_classification, Virology, Phenotype, immunity, United States, peritrophic matrix, Infectious Diseases

Abstract

Tsetse flies are the most important vectors of African trypanosomiasis but, surprisingly, are highly refractory to trypanosome parasite infection. In populations of wild caught flies, it is rare to find mature salivarian and mouthpart parasite infection rates exceeding 1 and 15%, respectively. This inherent refractoriness persists throughout the lifespan of the fly, although extreme starvation and suboptimal environmental conditions can cause a reversion to the susceptible phenotype. The teneral phenomenon is a phenotype unique to newly emerged, previously unfed tsetse, and is evidenced by a profound susceptibility to trypanosome infection. This susceptibility persists for only a few days post-emergence and decreases with fly age and bloodmeal acquisition. Researchers investigating trypanosome-tsetse interactions routinely exploit this phenomenon by using young, unfed (teneral) flies to naturally boost trypanosome establishment and maturation rates. A suite of factors may contribute, at least in part, to this unusual parasite permissive phenotype. These include the physical maturity of midgut barriers, the activation of immunoresponsive tissues and their effector molecules, and the role of the microflora within the midgut of the newly emerged fly. However, at present, the molecular mechanisms that underpin the teneral phenomenon still remain unknown. This review will provide a historical overview of the teneral phenomenon and will examine immune-related factors that influence, and may help us better understand, this unusual phenotype.

Published

2013

34. Tsetse EP protein protects the fly midgut from trypanosome establishment

Author

Terry W. Pearson, Stella Lehane, Lee R. Haines, and Michael J. Lehane

Subjects

lcsh:Immunologic diseases. Allergy, Tsetse Flies, Trypanosoma congolense, Molecular Sequence Data, Trypanosoma brucei brucei, Immunology/Innate Immunity, 030231 tropical medicine, Immunology, Trypanosoma brucei, Microbiology, 03 medical and health sciences, 0302 clinical medicine, Virology, parasitic diseases, Genetics, medicine, Animals, African trypanosomiasis, Amino Acid Sequence, RNA, Small Interfering, Molecular Biology, lcsh:QH301-705.5, RNA, Double-Stranded, 030304 developmental biology, 2. Zero hunger, 0303 health sciences, Base Sequence, biology, Host (biology), fungi, Tsetse fly, Midgut, biology.organism_classification, medicine.disease, 3. Good health, Cell biology, Gastrointestinal Tract, Trypanosomiasis, African, lcsh:Biology (General), Starvation, Gene Knockdown Techniques, Vector (epidemiology), Trypanosoma, Insect Proteins, Parasitology, lcsh:RC581-607, Trypanosomiasis, Research Article

Abstract

African trypanosomes undergo a complex developmental process in their tsetse fly vector before transmission back to a vertebrate host. Typically, 90% of fly infections fail, most during initial establishment of the parasite in the fly midgut. The specific mechanism(s) underpinning this failure are unknown. We have previously shown that a Glossina-specific, immunoresponsive molecule, tsetse EP protein, is up regulated by the fly in response to gram-negative microbial challenge. Here we show by knockdown using RNA interference that this tsetse EP protein acts as a powerful antagonist of establishment in the fly midgut for both Trypanosoma brucei brucei and T. congolense. We demonstrate that this phenomenon exists in two species of tsetse, Glossina morsitans morsitans and G. palpalis palpalis, suggesting tsetse EP protein may be a major determinant of vector competence in all Glossina species. Tsetse EP protein levels also decline in response to starvation of the fly, providing a possible explanation for increased susceptibility of starved flies to trypanosome infection. As starvation is a common field event, this fact may be of considerable importance in the epidemiology of African trypanosomiasis., Author Summary In Africa, tsetse flies transmit the trypanosomes causing the devastating diseases sleeping sickness in man and nagana in domesticated animals. These diseases are major causes of underdevelopment in Africa. Paradoxically, most, but not all, flies are resistant to infection with trypanosomes, but we do not have a clear picture of how flies fight off trypanosomes. Here we show that a particular, tsetse-specific immune responsive protein called tsetse EP acts as a powerful antagonist of trypanosome establishment in the fly midgut. It is known that starvation of flies leads to an increase in their susceptibility to trypanosomes and this may be a considerable factor in the epidemiology of the disease in Africa. Here we demonstrate that starvation leads to a decrease in tsetse EP levels, which may explain how starvation of the fly works to increase its susceptibility.

Published

2010

35. Chapter 3 The Enemy Within

Author

Deirdre Walshe, Cher-Pheng Ooi, Michael J. Lehane, and Lee R. Haines

Subjects

Entomology, biology, Endosymbiosis, Host (biology), fungi, Tsetse fly, Zoology, Domestication, biology.organism_classification, Genome, Symbiotic bacteria, Glossinidae

Abstract

Tsetse flies (Diptera: Glossinidae) are vectors of several species of African trypanosomes pathogenic to both man and his domesticated animals. The diseases they cause continue to have a devastating impact at the level of individual lives and the development of the entire African continent. Understanding the key molecular interactions between the trypanosome parasite and its tsetse fly host may enable more effective control strategies. We are now entering a new, exciting phase for such studies because four key trypanosome genomes are in the final stages of sequencing, assembly and annotation, the tsetse symbiont genomes are available and the Glossina genome is in the latter stages of sequencing. To exploit this information to its fullest extent it is essential that all groups of researchers, those studying trypanosomes, the symbionts and those studying tsetse flies, fully understand the biology of all component parts of the interaction. In addition there are very few entomology laboratories working in this area and more need to be recruited if discovery is to proceed at a good pace. To help achieve both aims, we here outline tsetse–trypanosome interactions from an entomological viewpoint. The trypanosome parasite faces a number of barriers to establishment, survival and maturation within the fly host. In particular, we describe how the tsetse midgut environment, the fly immune system and the fly's symbiotic bacteria contribute to these barriers.

Published

2009

36. Theileria

Author

Richard P. Bishop, David O. Odongo, David J. Mann, Terry W. Pearson, Chihiro Sugimoto, Lee R. Haines, Elizabeth Glass, Kirsty Jensen, Ulrike Seitzer, Jabbar S. Ahmed, Simon P. Graham, and Etienne P. de Villiers

Published

2009

37. Killing of trypanosomatid parasites by a modified bovine host defense peptide, BMAP-18

Author

Terry W. Pearson, Lee R. Haines, Brent E. Gowen, Angela M. Jackson, Brett A. Eyford, Robert E. W. Hancock, Jamie M. Thomas, Morteza Razavi, and Cristalle N. Watson

Subjects

Insecta, medicine.medical_treatment, Cell Biology/Cell Growth and Division, Cathelicidin, Mice, Parasitic Sensitivity Tests, Biochemistry/Protein Chemistry, 0303 health sciences, Mice, Inbred BALB C, biology, lcsh:Public aspects of medicine, Sodalis glossinidius, Flow Cytometry, Trypanocidal Agents, 3. Good health, Mitochondria, Infectious Diseases, Research Article, Sodalis, food.ingredient, lcsh:Arctic medicine. Tropical medicine, lcsh:RC955-962, Cell Survival, Antimicrobial peptides, Trypanosoma brucei brucei, Leishmania donovani, Trypanosoma brucei, Spodoptera, Cell Line, 03 medical and health sciences, food, Cell Line, Tumor, Immunology/Immunity to Infections, medicine, Animals, Humans, 030304 developmental biology, Infectious Diseases/Antimicrobials and Drug Resistance, 030306 microbiology, Tumor Necrosis Factor-alpha, Public Health, Environmental and Occupational Health, Proteins, lcsh:RA1-1270, biology.organism_classification, Leishmania, Virology, Rats, Microscopy, Fluorescence, Trypanosoma, Microscopy, Electron, Scanning, NIH 3T3 Cells, Antimicrobial Cationic Peptides, HeLa Cells

Abstract

Background Tropical diseases caused by parasites continue to cause socioeconomic devastation that reverberates worldwide. There is a growing need for new control measures for many of these diseases due to increasing drug resistance exhibited by the parasites and problems with drug toxicity. One new approach is to apply host defense peptides (HDP; formerly called antimicrobial peptides) to disease control, either to treat infected hosts, or to prevent disease transmission by interfering with parasites in their insect vectors. A potent anti-parasite effector is bovine myeloid antimicrobial peptide-27 (BMAP-27), a member of the cathelicidin family. Although BMAP-27 is a potent inhibitor of microbial growth, at higher concentrations it also exhibits cytotoxicity to mammalian cells. We tested the anti-parasite activity of BMAP-18, a truncated peptide that lacks the hydrophobic C-terminal sequence of the BMAP-27 parent molecule, an alteration that confers reduced toxicity to mammalian cells. Methodology/Principal Findings BMAP-18 showed strong growth inhibitory activity against several species and life cycle stages of African trypanosomes, fish trypanosomes and Leishmania parasites in vitro. When compared to native BMAP-27, the truncated BMAP-18 peptide showed reduced cytotoxicity on a wide variety of mammalian and insect cells and on Sodalis glossindius, a bacterial symbiont of the tsetse vector. The fluorescent stain rhodamine 123 was used in immunofluorescence microscopy and flow cytometry experiments to show that BMAP-18 at low concentrations rapidly disrupted mitochondrial potential without obvious alteration of parasite plasma membranes, thus inducing death by apoptosis. Scanning electron microscopy revealed that higher concentrations of BMAP-18 induced membrane lesions in the parasites as early as 15 minutes after exposure, thus killing them by necrosis. In addition to direct killing of parasites, BMAP-18 was shown to inhibit LPS-induced secretion of tumour necrosis factor alpha (TNF-α), a cytokine that is associated with inflammation and cachexia (wasting) in sleeping sickness patients. As a prelude to in vivo applications, high affinity antibodies to BMAP-18 were produced in rabbits and used in immuno-mass spectrometry assays to detect the intact peptide in human blood and plasma. Conclusions/Significance BMAP-18, a truncated form of the potent antimicrobial BMAP-27, showed low toxicity to mammalian cells, insect cells and the tsetse bacterial symbiont Sodalis glossinidius while retaining an ability to kill a variety of species and life cycle stages of pathogenic kinetoplastid parasites in vitro. BMAP-18 also inhibited secretion of TNF-α, an inflammatory cytokine that plays a role in the cachexia associated with African sleeping sickness. These findings support the idea that BMAP-18 should be explored as a candidate for therapy of economically important trypanosome-infected hosts, such as cattle, fish and humans, and for paratransgenic expression in Sodalis glossinidius, a bacterial symbiont in the tsetse vector, as a strategy for interference with trypanosome transmission., Author Summary Protozoan parasites cause serious diseases in large areas of the tropics. Control of these diseases depends to a great extent on the use of therapeutic drugs, many of which are highly toxic. In addition, parasite resistance to several of the front-line drugs is increasing. Host defense peptides (HDP; formerly called antimicrobial peptides) have recently received attention as potential anti-parasite effector molecules. We earlier reported that one such peptide, bovine myeloid antimicrobial peptide (BMAP-27), is a potent inhibitor of the growth of trypanosomes and Leishmania in vitro. Here we report our studies on BMAP-18, a truncated form of BMAP-27, which showed reduced toxicity to mammalian and insect cells and yet retained its direct toxicity to parasites in vitro. BMAP-18 also strongly inhibited LPS-induced release of tumour-necrosis factor alpha (TNF-α) from human leukocytes, and thus has immunomodulatory activity. These findings suggest that BMAP-18 has potential as a therapeutic agent for treatment of infected animals or as an inhibitor of parasite transmission by their insect vectors. In anticipation of using BMAP-18 in vivo, we have also developed high affinity antibodies to BMAP-18 and have shown that these can be used, in conjunction with mass spectrometry, to detect the peptide in whole blood or plasma.

Published

2008

38. Infections with immunogenic trypanosomes reduce tsetse reproductive fitness: potential impact of different parasite strains on vector population structure

Author

Lee R. Haines, Terry W. Pearson, Serap Aksoy, Jan Medlock, Changyun Hu, Nurper Guz, Amy F. Savage, Rita V. M. Rio, Dana Nayduch, Geoffrey M. Attardo, Alison P. Galvani, and Boelaert, Marleen

Subjects

Male, Trypanosoma brucei rhodesiense, Immunology/Innate Immunity, Protozoan Proteins, Microbiology/Innate Immunity, Medical and Health Sciences, 0302 clinical medicine, Parasite hosting, 2.2 Factors relating to the physical environment, Northern, Microbiology/Parasitology, Aetiology, 0303 health sciences, biology, Blotting, Reverse Transcriptase Polymerase Chain Reaction, lcsh:Public aspects of medicine, Reproduction, Biological Sciences, Fecundity, 3. Good health, Microbiology/Immunity to Infections, Infectious Diseases, Ecology/Population Ecology, Wigglesworthia, Female, Infection, Western, Research Article, lcsh:Arctic medicine. Tropical medicine, Tsetse Flies, lcsh:RC955-962, 030231 tropical medicine, Blotting, Western, Zoology, Parasitism, Host-Parasite Interactions, Vaccine Related, 03 medical and health sciences, Tropical Medicine, Immunology/Immunity to Infections, Animals, 030304 developmental biology, Host (biology), Prevention, fungi, Public Health, Environmental and Occupational Health, lcsh:RA1-1270, biology.organism_classification, Blotting, Northern, Vector-Borne Diseases, Good Health and Well Being, Fertility, Vector (epidemiology), Immunology, Immunology/Immune Response, Trypanosoma, Immunization

Abstract

The parasite Trypanosoma brucei rhodesiense and its insect vector Glossina morsitans morsitans were used to evaluate the effect of parasite clearance (resistance) as well as the cost of midgut infections on tsetse host fitness. Tsetse flies are viviparous and have a low reproductive capacity, giving birth to only 6–8 progeny during their lifetime. Thus, small perturbations to their reproductive fitness can have a major impact on population densities. We measured the fecundity (number of larval progeny deposited) and mortality in parasite-resistant tsetse females and untreated controls and found no differences. There was, however, a typanosome-specific impact on midgut infections. Infections with an immunogenic parasite line that resulted in prolonged activation of the tsetse immune system delayed intrauterine larval development resulting in the production of fewer progeny over the fly's lifetime. In contrast, parasitism with a second line that failed to activate the immune system did not impose a fecundity cost. Coinfections favored the establishment of the immunogenic parasites in the midgut. We show that a decrease in the synthesis of Glossina Milk gland protein (GmmMgp), a major female accessory gland protein associated with larvagenesis, likely contributed to the reproductive lag observed in infected flies. Mathematical analysis of our empirical results indicated that infection with the immunogenic trypanosomes reduced tsetse fecundity by 30% relative to infections with the non-immunogenic strain. We estimate that a moderate infection prevalence of about 26% with immunogenic parasites has the potential to reduce tsetse populations. Potential repercussions for vector population growth, parasite–host coevolution, and disease prevalence are discussed., Author Summary In many cases, parasites adapt to their hosts' biology over time and the extent of their harmful effects gradually diminishes. Insect-transmitted parasites such as African trypanosomes, however, are unusually pathogenic for their mammalian hosts because they rely on their invertebrate hosts for transmission to the next mammalian host. To ensure their maximum transmission, it is essential that parasite infections do not compromise insect host's fitness traits, including longevity and host-finding ability. Our results in tsetse indicate that, as theory predicts, trypanosome infections do not reduce host longevity. Instead, they divert host resources from reproduction and can reduce reproductive output by as much as 30%. Such loss of reproductive fitness occurs as a result of the induction of tsetse's immune responses. A closely related non-immunogenic parasite line does not induce host responses and does not compromise host fecundity. It is possible that host immune responses are needed in the case of the immunogenic line to control the parasite density to prevent excessive host damage. Because tsetse are viviparous and each adult female typically gives rise to only few progeny during their lifetime, even modest costs on reproduction can have a significant impact on host abundance. Our model predicts that if the prevalence of immunogenic parasite infections in tsetse populations reaches over 26%, they begin to have a negative impact on population growth rate. Infection rates as high as 30% have been reported with trypanosomes in the field. Our laboratory findings coupled with our modeling studies now provide a framework to investigate the status of co-infections, host immune activation processes, fecundity outcomes, transmission dynamics, and host virulence phenotypes in natural tsetse–trypanosome populations.

Published

2007

39. On the mechanism of mitochondrial uncoupling protein 1 function

Author

Eamon P. Breen, Richard K. Porter, Andrew Murphy, Sébastien G. Gouin, Lee R. Haines, Angela M. Jackson, Terry W. Pearson, and Paul V. Murphy

Subjects

Anions, Proteolipids, Molecular Sequence Data, Palmitic Acid, Mitochondrion, Biochemistry, Guanosine Diphosphate, Peptide Mapping, Cofactor, Ion Channels, Mass Spectrometry, Mitochondrial Proteins, Oxygen Consumption, Adipose Tissue, Brown, Brown adipose tissue, medicine, Escherichia coli, Animals, Amino Acid Sequence, Phosphorylation, Rats, Wistar, Molecular Biology, Uncoupling Protein 1, chemistry.chemical_classification, Ions, Liposome, biology, Chemistry, Uncoupling Agents, Fatty Acids, Fatty acid, Membrane Proteins, Cell Biology, Thermogenin, Recombinant Proteins, Mitochondria, Rats, medicine.anatomical_structure, Spectrometry, Fluorescence, Mechanism of action, Liposomes, biology.protein, Electrophoresis, Polyacrylamide Gel, medicine.symptom, Protons, Carrier Proteins, Flux (metabolism)

Abstract

Native uncoupling protein 1 (UCP 1) was purified from rat mitochondria by hydroxyapatite chromatography and identified by peptide mass mapping and tandem mass spectrometry. Native and expressed UCP 1 were reconstituted into liposomes, and proton flux through UCP 1 was shown to be fatty acid-dependent and GDP-sensitive. To investigate the mechanism of action of UCP 1, we determined whether hydrophilic modification of the omega-carbon of palmitate effected its transport function. We show that proton flux was greater through native UCP 1-containing proteoliposomes when facilitated by less hydrophilically modified palmitate (palmitateomega-methoxypalmitateomega-hydroxypalmitate with little or no proton flux due to glucose-O-omega-palmitate or undecanesulfonate). We show that non-proton-dependent charge transfer was greater when facilitated by less hydrophilically modified palmitate (palmitate/undecanesulfonateomega-methoxypalmitateomega-hydroxypalmitate, with no non-proton-dependent charge transfer flux due to glucose-O-omega-palmitate). We show that the GDP-inhibitable oxygen consumption rate in brown adipose tissue mitochondria was reversed by palmitate (as expected) but not by glucose-O-omega-palmitate. Our data are consistent with the model that UCP 1 flips long-chain fatty acid anions and contradict the "cofactor" model of UCP 1 function.

Published

2005

40. Analysis of the transcriptome of the protozoan Theileria parva using MPSS reveals that the majority of genes are transcriptionally active in the schizont stage

Author

Lee R. Haines, David C. Hoyle, Trushar Shah, Roger Pelle, Evans L. N. Taracha, Charles Lu, Simon P. Graham, Malcolm J. Gardner, Terry W. Pearson, Richard P. Bishop, Andy Brass, Helen Hulme, Simon Kang’a, Brian Hass, Owen White, Jennifer R. Wortman, Vishvanath Nene, and Etienne P. de Villiers

Subjects

Transcriptional Activation, Theileria parva, 030231 tropical medicine, Protozoan Proteins, Genomics, Genome, Article, Massively parallel signature sequencing, Transcriptome, 03 medical and health sciences, Open Reading Frames, 0302 clinical medicine, Complementary DNA, parasitic diseases, Genetics, Animals, RNA, Antisense, Gene, 030304 developmental biology, 0303 health sciences, biology, Sequence Analysis, RNA, Telomere, biology.organism_classification, Molecular biology, Open reading frame, Genome, Protozoan, RNA, Protozoan

Abstract

Massively parallel signature sequencing (MPSS) was used to analyze the transcriptome of the intracellular protozoan Theileria parva. In total 1,095,000, 20 bp sequences representing 4371 different signatures were generated from T.parva schizonts. Reproducible signatures were identified within 73% of potentially detectable predicted genes and 83% had signatures in at least one MPSS cycle. A predicted leader peptide was detected on 405 expressed genes. The quantitative range of signatures was 4-52,256 transcripts per million (t.p.m.). Rare transcripts (

Published

2005

41. Identification of a functioning mitochondrial uncoupling protein 1 in thymus

Author

Lee R. Haines, Eamon P. Breen, Terry W. Pearson, Clare M. Brennan, A.M. Carroll, Richard K. Porter, Caitriona M. Walsh, and Padraic G. Fallon

Subjects

Molecular Sequence Data, Thymus Gland, Mitochondrion, Biology, Tandem mass spectrometry, Biochemistry, Guanosine Diphosphate, Antibodies, Ion Channels, Mitochondrial Proteins, Mice, Brown adipose tissue, medicine, Uncoupling protein, Animals, Amino Acid Sequence, RNA, Messenger, Rats, Wistar, Molecular Biology, Peptide sequence, GeneralLiterature_REFERENCE(e.g.,dictionaries,encyclopedias,glossaries), Uncoupling Protein 1, Mice, Knockout, Reverse Transcriptase Polymerase Chain Reaction, RNA, Membrane Proteins, Cell Biology, Thermogenin, Mitochondria, Rats, Mice, Inbred C57BL, medicine.anatomical_structure, Female, Clinical Medicine, Carrier Proteins, Flux (metabolism)

Abstract

PUBLISHED, We present evidence that rat and mouse thymi contain mitochondrial uncoupling protein (UCP 1). Reverse transcriptase-PCR detected RNA transcripts for UCP 1 in whole thymus and in thymocytes. Furthermore, using antibodies to UCP 1 the protein was also detected in mitochondria isolated from whole thymus and thymocytes but not in thymus mitochondria from UCP 1 knock-out mice. Evidence for functional UCP 1 in thymus mitochondria was obtained by a comparative analysis with the kinetics of GDP binding in mitochondria from brown adipose tissue. Both tissues showed equivalent Bmax and KD values. In addition, a large component of the nonphosphorylating oxygen consumption by thymus mitochondria was inhibited by GDP and subsequently stimulated by addition of nanomolar concentrations of palmitate. UCP 1 was purified from thymus mitochondria by hydroxyapatite chromatography. The isolated protein was identified by peptide mass mapping and tandem mass spectrometry by using MALDI-TOF and LC-MS/MS, respectively. We conclude that the thymus contains a functioning UCP 1 that has the capacity to regulate metabolic flux and production of reactive oxygen-containing molecules in the thymus.

Published

2005

42. Identification of midgut proteins that are differentially expressed in trypanosome-susceptible and normal tsetse flies (Glossina morsitans morsitans)

Author

Robert W. Olafson, Terry W. Pearson, J D Haddow, Lee R. Haines, and R. H. Gooding

Subjects

Trypanosoma, Proteome, Tsetse Flies, Mutant, Molecular Sequence Data, Genes, Insect, Biochemistry, parasitic diseases, Parasite hosting, Animals, Amino Acid Sequence, Molecular Biology, Gene, Two-dimensional gel electrophoresis, biology, fungi, Wild type, Midgut, biology.organism_classification, Molecular biology, Cell biology, Gene Expression Regulation, Insect Science, Insect Proteins, Digestive System

Abstract

Molecules in the midgut of tsetse flies (Diptera: Glossinidiae) are thought to play important roles in the life cycle of African trypanosomes by influencing initial parasite establishment and subsequent differentiation events that ultimately lead to maturation of mammal-infective trypanosomes. The molecular composition of the tsetse midgut is, therefore, of critical importance to disease transmission by these medically important vectors. In this study we compared protein expression profiles of midguts of the salmon mutant and wild type Glossina morsitans morsitans Westwood that display marked differences in their susceptibility to infection by African trypanosomes. Isotope coded affinity tag (ICAT) technology was used to identify 207 proteins including 17 that were up regulated and nine that were down regulated in the salmon mutants. Several of the up regulated molecules were previously described as tsetse midgut or salivary gland proteins. Of particular interest was the up regulation in the salmon flies of tsetse midgut EP protein, a recently described molecule with lectin-like activity that was also found to be induced in tsetse by bacterial challenge. The up regulation of the EP protein in midguts of salmon mutants was confirmed by two-dimensional gel electrophoresis and tandem mass spectrometry.

Published

2004

43. An effective and rapid method for functional characterization of immunoadsorbents using POROS beads and flow cytometry

Author

N Leigh, Anderson, Lee R, Haines, and Terry W, Pearson

Subjects

Chromatography, Flow Cytometry, Antibodies, Mass Spectrometry, Protein Structure, Tertiary, Hydrazines, Animals, Humans, Rabbits, Antigens, Coloring Agents, Immunosorbents, Peptides, Protein Binding

Abstract

To facilitate the construction, functional characterization, and use of immunoadsorbents, we have developed a flow cytometry method that allows rapid assessment of large numbers of particle-bound antibodies. Protein G derivitized POROS beads were used to bind affinity-purified antibodies specific for synthetic peptides designed from human plasma proteins. The antibodies were covalently coupled to the beads and used to capture and release synthetic peptides that had been labeled at the C-terminus with the fluorochrome Alexa Fluor 488. Antibody coupling and specificity of antigen binding and release were measured by analysis of the POROS affinity beads by flow cytometry. The affinity-capture matrixes were also used through several antigen-binding and release cycles without loss of peptide binding efficiency. The ability to produce and characterize extremely small amounts of POROS affinity matrices will facilitate their use in protein microchemical procedures such as protein chip technology, monoclonal antibody screening and mass spectrometry, applications where analytes are limiting or present in low abundance in complex mixtures.

Published

2004

44. Proteome analysis of abundantly expressed proteins from unfed larvae of the cattle tick, Boophilus microplus

Author

P.M. Untalan, Lee R. Haines, Terry W. Pearson, and Felix D. Guerrero

Subjects

Proteomics, Ixodidae, Proteome, Molecular Sequence Data, Gene Expression, Peptide, Biology, Biochemistry, Heat shock protein, Animals, Electrophoresis, Gel, Two-Dimensional, Amino Acid Sequence, Molecular Biology, Peptide sequence, chemistry.chemical_classification, Gel electrophoresis, Two-dimensional gel electrophoresis, Binding protein, Molecular biology, chemistry, Insect Science, Larva, Insect Proteins, Sequence Alignment

Abstract

Protein expression in unfed larvae of the cattle tick, Boophilus microplus, was characterized using gel electrophoresis and mass spectrometry in an effort to assemble a database of proteins produced at this stage of development. Soluble and insoluble proteins were extracted and resolved by two-dimensional (2D) gel electrophoresis. Twenty abundantly expressed larval proteins were selected for peptide mass mapping and for peptide sequencing by matrix-assisted laser desorption/ionization time-of-flight (MALDI-ToF) and quadrupole time-of-flight (Q-ToF) tandem mass spectrometry (MS), respectively. Only one protein, tropomyosin, was unequivocally identified from its peptide mass map. Ten proteins were assigned putative identities based on BLAST searching of heterologous databases with peptide sequences. These included a cytoskeletal protein (troponin I), multiple cuticular proteins, a glycine-rich salivary gland-associated protein and proteins with a presumed housekeeping role (arginine kinase, a high-mobility group protein and a small heat shock protein). Eight additional proteins were identified by searching translated open reading frames of a B. microplus EST database (unpublished): putative fatty-acid binding protein, thioredoxin, glycine-rich salivary gland protein and additional cuticular proteins. One remaining protein was not identifiable, suggesting it may be a novel molecule. The ongoing assembly of this database contributes to our understanding of proteins expressed by the tick and provides a resource that can be mined for molecules that play a role in tick-host interactions.

Published

2004

45. The relationship between flesh quality and numbers of Kudoa thyrsites plasmodia and spores in farmed Atlantic salmon, Salmo salar L

Author

M H Booy, Terry W. Pearson, Robert W. Olafson, D. J. Whitaker, C L Falkenberg, V Funk, Lee R. Haines, J C Chase, and J A Dawson-Coates

Subjects

Quality Control, Veterinary medicine, Meat, Veterinary (miscellaneous), Salmo salar, Spores, Protozoan, Aquaculture, Aquatic Science, Myxosporea, Fish Diseases, Food Parasitology, Animals, Salmo, Kudoa thyrsites, Fillet (mechanics), Protozoan Infections, Animal, Myxozoa, biology, business.industry, Flesh, Eukaryota, Anatomy, biology.organism_classification, Spore, business

Abstract

Atlantic salmon, Salmo salar L., were exposed to Kudoa thyrsites (Myxozoa, Myxosporea)-containing sea water for 15 months, and then harvested and assessed for parasite burden and fillet quality. At harvest, parasites were enumerated in muscle samples from a variety of somatic and opercular sites, and mean counts were determined for each fish. After 6 days storage at 4 degrees C, fillet quality was determined by visual assessment and by analysis of muscle firmness using a texture analyzer. Fillet quality could best be predicted by determining mean parasite numbers and spore counts in all eight tissue samples (somatic and opercular) or in four fillet samples, as the counts from opercular samples alone showed greater variability and thus decreased reliability. The variability in both plasmodia and spore numbers between tissue samples taken from an individual fish indicated that the parasites were not uniformly distributed in the somatic musculature. Therefore, to best predict the probable level of fillet degradation caused by K. thyrsites infections, multiple samples must be taken from each fish. If this is performed, a mean plasmodia count of 0.3 mm(-2) or a mean spore count of 4.0 x 10(5) g(-1) of tissue are the levels where the probability of severe myoliquefaction becomes a significant risk.

Published

2003

46. Immunological detection of Kudoa thyrsites spores in muscle tissues of farmed Atlantic salmon, Salmo salar L

Author

J A Dawson-Coates, Robert W. Olafson, D. J. Whitaker, Lee R. Haines, J C Chase, Terry W. Pearson, J D Haddow, and M H Booy

Subjects

biology, Veterinary (miscellaneous), Immunoblotting, Salmo salar, Spores, Protozoan, Zoology, Eukaryota, Fluorescent Antibody Technique, Aquatic Science, biology.organism_classification, Spore, Fishery, Fish Diseases, Animals, Salmo, Kudoa thyrsites, Muscle, Skeletal, Protozoan Infections, Animal

Published

2003

47. Identification of major soluble salivary gland proteins in teneral Glossina morsitans morsitans

Author

Serap Aksoy, R. H. Gooding, Brett A. D. Poulis, Terry W. Pearson, Lee R. Haines, and J D Haddow

Subjects

Gel electrophoresis, chemistry.chemical_classification, Salivary gland, Tsetse Flies, Biology, Tandem mass spectrometry, Proteomics, Mass spectrometry, Biochemistry, Molecular biology, Mass Spectrometry, Salivary Glands, Amino acid, Matrix-assisted laser desorption/ionization, medicine.anatomical_structure, chemistry, Solubility, Insect Science, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, medicine, Animals, Insect Proteins, Molecular Biology, Gene, Chromatography, High Pressure Liquid

Abstract

Salivary glands of tsetse flies (Diptera: Glossinidiae) contain molecules that are involved in preventing blood clotting during feeding as well as molecules thought to be intimately associated with trypanosome development and maturation. Here we present a protein microchemical analysis of the major soluble proteins of the salivary glands of Glossina morsitans morsitans, an important vector of African trypanosomes. Differential solubilization of salivary proteins was followed by reverse-phase, high-performance liquid chromatography (HPLC) and analysis of fractions by 1-D gel electrophoresis to reveal four major proteins. Each protein was subjected to amino acid microanalysis and N-terminal microsequencing. A protein chemical approach using high-resolution 2-D gel electrophoresis and mass spectrometry was also used to identify the salivary proteins. Matrix-assisted, laser desorption ionization time-of-flight (MALDI-TOF) mass spectrometry and quadrupole time-of-flight (Q-TOF) tandem mass spectrometry methods were used for peptide mass mapping and sequencing, respectively. Sequence information and peptide mass maps queried against the NCBI non-redundant database confirmed the identity of the first protein as tsetse salivary gland growth factor-1 (TSGF-1). Two proteins with no known function were identified as tsetse salivary gland protein 1 (Tsal 1) and tsetse salivary gland protein 2 (Tsal 2). The fourth protein was identified as Tsetse antigen-5 (TAg-5), which is a member of a large family of anti-haemostatic proteins. The results show that these four proteins are the most abundant soluble gene products present in salivary glands of teneral G. m. morsitans. We discuss the possible functions of these major proteins in cyclical transmission of African trypanosomes.

Published

2002

48. Post Eclosion Age Predicts the Prevalence of Midgut Trypanosome Infections in Glossina

Author

Michael J. Lehane, Lee R. Haines, and Deirdre Walshe

Subjects

Male, Trypanosoma congolense, lcsh:Medicine, Insect, Global Health, 0302 clinical medicine, Prevalence, Parasite hosting, lcsh:Science, media_common, 0303 health sciences, Multidisciplinary, biology, Age Factors, Infectious Diseases, Medicine, Female, Disease Susceptibility, Research Article, Tsetse Flies, Infectious Disease Control, media_common.quotation_subject, Trypanosoma brucei brucei, 030231 tropical medicine, Microbiology, Vector Biology, African Trypanosomiasis, 03 medical and health sciences, Trypanosomiasis, parasitic diseases, Parasitic Diseases, medicine, Animals, Animal Physiology, Biology, 030304 developmental biology, Parasitic life cycles, lcsh:R, fungi, Parasite Physiology, Tsetse fly, Vectors and Hosts, Midgut, biology.organism_classification, medicine.disease, Virology, Insect Vectors, Vector (epidemiology), Trypanosoma, Parasitology, lcsh:Q, Digestive System, Zoology, Entomology

Abstract

The teneral phenomenon, as observed in Glossina sp., refers to the increased susceptibility of the fly to trypanosome infection when the first bloodmeal taken is trypanosome-infected. In recent years, the term teneral has gradually become synonymous with unfed, and thus fails to consider the age of the newly emerged fly at the time the first bloodmeal is taken. Furthermore, conflicting evidence exists of the effect of the age of the teneral fly post eclosion when it is given the infected first bloodmeal in determining the infection prevalence. This study demonstrates that it is not the feeding history of the fly but rather the age (hours after eclosion of the fly from the puparium) of the fly when it takes the first (infective) bloodmeal that determines the level of fly susceptibility to trypanosome infection. We examine this phenomenon in male and female flies from two distinct tsetse clades (Glossina morsitans morsitans and Glossina palpalis palpalis) infected with two salivarian trypanosome species, Trypanosoma (Trypanozoon) brucei brucei and Trypanosoma (Nannomonas) congolense using Fisher's exact test to examine differences in infection rates. Teneral tsetse aged less than 24 hours post-eclosion (h.p.e.) are twice as susceptible to trypanosome infection as flies aged 48 h.p.e. This trend is conserved across sex, vector clade and parasite species. The life cycle stage of the parasite fed to the fly (mammalian versus insect form trypanosomes) does not alter this age-related bias in infection. Reducing the numbers of parasites fed to 48 h.p.e., but not to 24 h.p.e. flies, increases teneral refractoriness. The importance of this phenomenon in disease biology in the field as well as the necessity of employing flies of consistent age in laboratory-based infection studies is discussed.

Published

2011

49. Cationic Antimicrobial Peptide Killing of African Trypanosomes and Sodalis glossinidius, a Bacterial Symbiont of the Insect Vector of Sleeping Sickness.

Author

Lee R. Haines, Robert E. W. Hancock, and Terry W. Pearson

Published

2003

50. Immunodetection of UCP1 in rat thymocytes

Author

Richard K. Porter, A.M. Carroll, Eamon P. Breen, Lee R. Haines, Clare M. Brennan, and Terry W. Pearson

Subjects

Immunoassay, biology, Connective tissue, Membrane Proteins, Thymus Gland, Mitochondrion, Biochemistry, Molecular biology, Thermogenin, Ion Channels, Rats, Mitochondrial Proteins, medicine.anatomical_structure, Immunoblot Analysis, biology.protein, medicine, Animals, Electrophoresis, Polyacrylamide Gel, Antibody, Rats, Wistar, Carrier Proteins, Uncoupling Protein 1

Abstract

Thymi were dissected from rats and connective tissue was removed. Mitochondria were purified from isolated thymocytes and immunoblot analysis was performed using an antibody specific for uncoupling protein 1, which detected a 32.5 kDa protein associated with mitochondria from the thymocytes. This implies that rat thymocytes contain uncoupling protein 1.