Your search keyword '"Leguia M"' showing total 37 results

1. Feasibility and effectiveness of a brief, intensive phylogenetics workshop in a middle-income country

Author

Pollett, S., Leguia, M., Nelson, M.I., Maljkovic Berry, I., Rutherford, G., Bausch, D.G., Kasper, M., Jarman, R., and Melendrez, M.

Published

2016

2. Efficacy of a spatial repellent for control of Aedes -borne virus transmission: A cluster-randomized trial in Iquitos, Peru

Author

Jenkins Sa, Leguia M, John P. Grieco, del Aguila C, Isabel Bazan, Escobedo-Vargas K, Christopher M. Barker, Silva Me, A. C. Morrison, Robert C. Reiner, Nicole L. Achee, Kawiecki Ab, Valerie A. Paz-Soldan, Helvio Astete, Guevara C, Robert D. Hontz, Barrera P, Flores-Mendoza C, Crystyan Siles, Huaman Aa, Thomas W. Scott, Abente Ej, Elson Wh, Campbell Wr, Gissella M. Vásquez, and Neil F. Lobo

Subjects

Aedes, education.field_of_study, Veterinary medicine, Multidisciplinary, biology, Population, Aedes aegypti, medicine.disease, biology.organism_classification, Dengue fever, chemistry.chemical_compound, Transfluthrin, chemistry, Vector (epidemiology), medicine, Clinical endpoint, Seroconversion, education

Abstract

Over half the world’s population is at risk for viruses transmitted by Aedes mosquitoes, such as, dengue and Zika. The primary vector, Aedes aegypti, thrives in urban environments. Despite decades of effort, cases and geographic range of Aedes-borne viruses (ABV) continue to expand. Rigorously proven vector control interventions that measure protective efficacy against ABV diseases is limited to Wolbachia in a single trial in Indonesia, and do not include any chemical intervention. Spatial repellents, a new option for efficient deployment, are designed to decrease human exposure to ABV by releasing active ingredients into the air that disrupt mosquito-human contact. A parallel, cluster-randomized controlled trial was conducted in Iquitos, Peru to quantify the impact of a transfluthrin-based spatial repellent on human ABV infection. From 2,907 households across 26 clusters (13 per arm), 1,578 participants were assessed for seroconversion (primary endpoint) by survival analysis. Incidence of acute disease was calculated among 16,683 participants (secondary endpoint). Adult mosquito collections were conducted to compare Ae. aegypti abundance, blood-fed rate and parity status through mixed effect difference-in-difference analyses. The spatial repellent significantly reduced ABV infection by 34·1% (1-sided 95% CI lower limit, 6·9%; 1-sided p-value=0·0236, z=1·98). Aedes aegypti abundance and blood-fed rates were significantly reduced by 28·6% (95% CI 24·1%, ∞); z=-9·11) and 12·4% (95% CI 4·2%, ∞); z=-2·43), respectively. Our trial provides the first conclusive statistical evidence from a pre-planned cluster randomized controlled clinical trial with a pre-defined effect size on the primary endpoint that was appropriate powered to prospectively quantify and statistically test for a difference in the impact of a chemical intervention, in this case a spatial repellent, to reduce the risk of ABV transmission compared to a placebo.Significance StatementVector interventions are needed for Aedes-borne viral diseases (dengue, Zika, chikungunya, and yellow fever) prevention, but their application is hindered by the lack of evidence proving they prevent infection or disease. Our research reports the first conclusive statistical evidence from a pre-planned, prospective cluster-randomized, controlled clinical trial (cRCT) of significant protective efficacy (34.1% hazard estimate) against human Aedes-borne virus (ABV) infection by a chemical-based vector control intervention, the most commonly used intervention category among all ABV World Health Organization recommendations. A previous trial against malaria in Indonesia indicated a positive trend but did not detect a significant effect. Results from our ABV study will help guide public health authorities responsible for operational management and world-wide prevention of ABV, and incentivize new strategies for disease prevention.

Published

2022

3. Prevalencia de la hipertensión arterial en poblaciones rurales del norte argentino

Author

De All, J., Lanfranconi, M., Bledel, I., Doval, H., Hughes, A., Laroti, A., Sánchez Aramburu, V., Gnocchi, D., Dubra, L., Gorosito, F., Henry, N., Leguia, M., Francos, J., González Viana, H., Saavedra, F., and Gnocchi, C.

Published

2012

4. 2ab assembly: a methodology for automatable, high-throughput assembly of standard biological parts

Author

Leguia Mariana, Brophy Jennifer AN, Densmore Douglas, Asante Angel, and Anderson J Christopher

Subjects

2ab reaction, Automated assembly, DNA fabrication, Synthetic biology, Biology (General), QH301-705.5

Abstract

Abstract There is growing demand for robust DNA assembly strategies to quickly and accurately fabricate genetic circuits for synthetic biology. One application of this technology is reconstitution of multi-gene assemblies. Here, we integrate a new software tool chain with 2ab assembly and show that it is robust enough to generate 528 distinct composite parts with an error-free success rate of 96%. Finally, we discuss our findings in the context of its implications for biosafety and biosecurity.

Published

2013

5. BglBricks: A flexible standard for biological part assembly

Author

Dueber John E, Anderson J Christopher, Leguia Mariana, Wu Gabriel C, Goler Jonathan A, Arkin Adam P, and Keasling Jay D

Subjects

Biology (General), QH301-705.5

Abstract

Abstract Background Standard biological parts, such as BioBricks™ parts, provide the foundation for a new engineering discipline that enables the design and construction of synthetic biological systems with a variety of applications in bioenergy, new materials, therapeutics, and environmental remediation. Although the original BioBricks™ assembly standard has found widespread use, it has several shortcomings that limit its range of potential applications. In particular, the system is not suitable for the construction of protein fusions due to an unfavorable scar sequence that encodes an in-frame stop codon. Results Here, we present a similar but new composition standard, called BglBricks, that addresses the scar translation issue associated with the original standard. The new system employs BglII and BamHI restriction enzymes, robust cutters with an extensive history of use, and results in a 6-nucleotide scar sequence encoding glycine-serine, an innocuous peptide linker in most protein fusion applications. We demonstrate the utility of the new standard in three distinct applications, including the construction of constitutively active gene expression devices with a wide range of expression profiles, the construction of chimeric, multi-domain protein fusions, and the targeted integration of functional DNA sequences into specific loci of the E. coli genome. Conclusions The BglBrick standard provides a new, more flexible platform from which to generate standard biological parts and automate DNA assembly. Work on BglBrick assembly reactions, as well as on the development of automation and bioinformatics tools, is currently underway. These tools will provide a foundation from which to transform genetic engineering from a technically intensive art into a purely design-based discipline.

Published

2010

6. A new lineage nomenclature to aid genomic surveillance of dengue virus.

Author

Hill V, Cleemput S, Pereira JS, Gifford RJ, Fonseca V, Tegally H, Brito AF, Ribeiro G, de Souza VC, Brcko IC, Ribeiro IS, De Lima ITT, Slavov SN, Sampaio SC, Elias MC, Tran VT, Kien DTH, Huynh T, Yacoub S, Dieng I, Salvato R, Wallau GL, Gregianini TS, Godinho FMS, Vogels CBF, Breban MI, Leguia M, Jagtap S, Roy R, Hapuarachchi C, Mwanyika G, Giovanetti M, Alcantara LCJ, Faria NR, Carrington CVF, Hanley KA, Holmes EC, Dumon W, Lima ARJ, Oliveira T, and Grubaugh ND

Subjects

Humans, Genotype, Genomics methods, Genetic Variation, Terminology as Topic, Dengue Virus genetics, Dengue Virus classification, Phylogeny, Genome, Viral, Dengue virology, Dengue epidemiology

Abstract

Dengue virus (DENV) is currently causing epidemics of unprecedented scope in endemic settings and expanding to new geographical areas. It is therefore critical to track this virus using genomic surveillance. However, the complex patterns of viral genomic diversity make it challenging to use the existing genotype classification system. Here, we propose adding 2 sub-genotypic levels of virus classification, named major and minor lineages. These lineages have high thresholds for phylogenetic distance and clade size, rendering them stable between phylogenetic studies. We present assignment tools to show that the proposed lineages are useful for regional, national, and subnational discussions of relevant DENV diversity. Moreover, the proposed lineages are robust to classification using partial genome sequences. We provide a standardized neutral descriptor of DENV diversity with which we can identify and track lineages of potential epidemiological and/or clinical importance. Information about our lineage system, including methods to assign lineages to sequence data and propose new lineages, can be found at: dengue-lineages.org., Competing Interests: I have read the journal’s policy and the authors of this manuscript have the following competing interests: SC and WD are affiliated with emweb. NDG is a paid consultant for BioNTech., (Copyright: © 2024 Hill et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.)

Published

2024

7. Highly pathogenic avian influenza A (H5N1) in marine mammals and seabirds in Peru.

Author

Leguia M, Garcia-Glaessner A, Muñoz-Saavedra B, Juarez D, Barrera P, Calvo-Mac C, Jara J, Silva W, Ploog K, Amaro L, Colchao-Claux P, Johnson CK, Uhart MM, Nelson MI, and Lescano J

Subjects

Animals, Humans, Peru epidemiology, Birds, Cetacea, Influenza in Birds epidemiology, Influenza A Virus, H5N1 Subtype genetics, Influenza, Human, Caniformia, Influenza A virus

Abstract

Highly pathogenic avian influenza (HPAI) A/H5N1 viruses (lineage 2.3.4.4b) are rapidly invading the Americas, threatening wildlife, poultry, and potentially evolving into the next global pandemic. In November 2022 HPAI arrived in Peru, triggering massive pelican and sea lion die-offs. We report genomic characterization of HPAI/H5N1 in five species of marine mammals and seabirds (dolphins, sea lions, sanderlings, pelicans and cormorants). Peruvian viruses belong to lineage 2.3.4.4b, but they are 4:4 reassortants where 4 genomic segments (PA, HA, NA and MP) position within the Eurasian lineage that initially entered North America from Eurasia, while the other 4 genomic segments (PB2, PB1, NP and NS) position within the American lineage (clade C) that circulated in North America. These viruses are rapidly accruing mutations, including mutations of concern, that warrant further examination and highlight an urgent need for active local surveillance to manage outbreaks and limit spillover into other species, including humans., (© 2023. Springer Nature Limited.)

Published

2023

8. Direct mosquito feedings on dengue-2 virus-infected people reveal dynamics of human infectiousness.

Author

Lambrechts L, Reiner RC Jr, Briesemeister MV, Barrera P, Long KC, Elson WH, Vizcarra A, Astete H, Bazan I, Siles C, Vilcarromero S, Leguia M, Kawiecki AB, Perkins TA, Lloyd AL, Waller LA, Kitron U, Jenkins SA, Hontz RD, Campbell WR, Carrington LB, Simmons CP, Ampuero JS, Vasquez G, Elder JP, Paz-Soldan VA, Vazquez-Prokopec GM, Rothman AL, Barker CM, Scott TW, and Morrison AC

Subjects

Animals, Humans, Viremia, Zika Virus Infection epidemiology, Zika Virus, Culicidae, Dengue epidemiology

Abstract

Dengue virus (DENV) transmission from humans to mosquitoes is a poorly documented, but critical component of DENV epidemiology. Magnitude of viremia is the primary determinant of successful human-to-mosquito DENV transmission. People with the same level of viremia, however, can vary in their infectiousness to mosquitoes as a function of other factors that remain to be elucidated. Here, we report on a field-based study in the city of Iquitos, Peru, where we conducted direct mosquito feedings on people naturally infected with DENV and that experienced mild illness. We also enrolled people naturally infected with Zika virus (ZIKV) after the introduction of ZIKV in Iquitos during the study period. Of the 54 study participants involved in direct mosquito feedings, 43 were infected with DENV-2, two with DENV-3, and nine with ZIKV. Our analysis excluded participants whose viremia was detectable at enrollment but undetectable at the time of mosquito feeding, which was the case for all participants with DENV-3 and ZIKV infections. We analyzed the probability of onward transmission during 50 feeding events involving 27 participants infected with DENV-2 based on the presence of infectious virus in mosquito saliva 7-16 days post blood meal. Transmission probability was positively associated with the level of viremia and duration of extrinsic incubation in the mosquito. In addition, transmission probability was influenced by the day of illness in a non-monotonic fashion; i.e., transmission probability increased until 2 days after symptom onset and decreased thereafter. We conclude that mildly ill DENV-infected humans with similar levels of viremia during the first two days after symptom onset will be most infectious to mosquitoes on the second day of their illness. Quantifying variation within and between people in their contribution to DENV transmission is essential to better understand the biological determinants of human infectiousness, parametrize epidemiological models, and improve disease surveillance and prevention strategies., Competing Interests: The authors have declared that no competing interests exist., (Copyright: This is an open access article, free of all copyright, and may be freely reproduced, distributed, transmitted, modified, built upon, or otherwise used by anyone for any lawful purpose. The work is made available under the Creative Commons CC0 public domain dedication.)

Published

2023

9. Quantifying heterogeneities in arbovirus transmission: Description of the rationale and methodology for a prospective longitudinal study of dengue and Zika virus transmission in Iquitos, Peru (2014-2019).

Author

Morrison AC, Paz-Soldan VA, Vazquez-Prokopec GM, Lambrechts L, Elson WH, Barrera P, Astete H, Briesemeister V, Leguia M, Jenkins SA, Long KC, Kawiecki AB, Reiner RC Jr, Perkins TA, Lloyd AL, Waller LA, Hontz RD, Stoddard ST, Barker CM, Kitron U, Elder JP, Rothman AL, and Scott TW

Subjects

Humans, Longitudinal Studies, Prospective Studies, Peru epidemiology, Zika Virus, Dengue Virus, Dengue, Zika Virus Infection epidemiology, Arboviruses

Abstract

Current knowledge of dengue virus (DENV) transmission provides only a partial understanding of a complex and dynamic system yielding a public health track record that has more failures than successes. An important part of the problem is that the foundation for contemporary interventions includes a series of longstanding, but untested, assumptions based on a relatively small portion of the human population; i.e., people who are convenient to study because they manifest clinically apparent disease. Approaching dengue from the perspective of people with overt illness has produced an extensive body of useful literature. It has not, however, fully embraced heterogeneities in virus transmission dynamics that are increasingly recognized as key information still missing in the struggle to control the most important insect-transmitted viral infection of humans. Only in the last 20 years have there been significant efforts to carry out comprehensive longitudinal dengue studies. This manuscript provides the rationale and comprehensive, integrated description of the methodology for a five-year longitudinal cohort study based in the tropical city of Iquitos, in the heart of the Peruvian Amazon. Primary data collection for this study was completed in 2019. Although some manuscripts have been published to date, our principal objective here is to support subsequent publications by describing in detail the structure, methodology, and significance of a specific research program. Our project was designed to study people across the entire continuum of disease, with the ultimate goal of quantifying heterogeneities in human variables that affect DENV transmission dynamics and prevention. Because our study design is applicable to other Aedes transmitted viruses, we used it to gain insights into Zika virus (ZIKV) transmission when during the project period ZIKV was introduced and circulated in Iquitos. Our prospective contact cluster investigation design was initiated by detecttion of a person with a symptomatic DENV infection and then followed that person's immediate contacts. This allowed us to monitor individuals at high risk of DENV infection, including people with clinically inapparent and mild infections that are otherwise difficult to detect. We aimed to fill knowledge gaps by defining the contribution to DENV transmission dynamics of (1) the understudied majority of DENV-infected people with inapparent and mild infections and (2) epidemiological, entomological, and socio-behavioral sources of heterogeneity. By accounting for factors underlying variation in each person's contribution to transmission we sought to better determine the type and extent of effort needed to better prevent virus transmission and disease., Competing Interests: The authors have declared that no competing interests exist., (Copyright: This is an open access article, free of all copyright, and may be freely reproduced, distributed, transmitted, modified, built upon, or otherwise used by anyone for any lawful purpose. The work is made available under the Creative Commons CC0 public domain dedication.)

Published

2023

10. Efficacy of a spatial repellent for control of Aedes -borne virus transmission: A cluster-randomized trial in Iquitos, Peru.

Author

Morrison AC, Reiner RC Jr, Elson WH, Astete H, Guevara C, Del Aguila C, Bazan I, Siles C, Barrera P, Kawiecki AB, Barker CM, Vasquez GM, Escobedo-Vargas K, Flores-Mendoza C, Huaman AA, Leguia M, Silva ME, Jenkins SA, Campbell WR, Abente EJ, Hontz RD, Paz-Soldan VA, Grieco JP, Lobo NF, Scott TW, and Achee NL

Subjects

Adult, Animals, Dengue epidemiology, Dengue prevention & control, Humans, Peru epidemiology, Zika Virus, Zika Virus Infection, Aedes, Insect Repellents, Mosquito Control standards, Mosquito Vectors, Vector Borne Diseases epidemiology, Vector Borne Diseases prevention & control, Vector Borne Diseases transmission

Abstract

Over half the world's population is at risk for viruses transmitted by Aedes mosquitoes, such as dengue and Zika. The primary vector, Aedes aegypti , thrives in urban environments. Despite decades of effort, cases and geographic range of Aedes -borne viruses (ABVs) continue to expand. Rigorously proven vector control interventions that measure protective efficacy against ABV diseases are limited to Wolbachia in a single trial in Indonesia and do not include any chemical intervention. Spatial repellents, a new option for efficient deployment, are designed to decrease human exposure to ABVs by releasing active ingredients into the air that disrupt mosquito-human contact. A parallel, cluster-randomized controlled trial was conducted in Iquitos, Peru, to quantify the impact of a transfluthrin-based spatial repellent on human ABV infection. From 2,907 households across 26 clusters (13 per arm), 1,578 participants were assessed for seroconversion (primary endpoint) by survival analysis. Incidence of acute disease was calculated among 16,683 participants (secondary endpoint). Adult mosquito collections were conducted to compare Ae. aegypti abundance, blood-fed rate, and parity status through mixed-effect difference-in-difference analyses. The spatial repellent significantly reduced ABV infection by 34.1% (one-sided 95% CI lower limit, 6.9%; one-sided P value = 0.0236, z = 1.98). Aedes aegypti abundance and blood-fed rates were significantly reduced by 28.6 (95% CI 24.1%, ∞); z = -9.11) and 12.4% (95% CI 4.2%, ∞); z = -2.43), respectively. Our trial provides conclusive statistical evidence from an appropriately powered, preplanned cluster-randomized controlled clinical trial of the impact of a chemical intervention, in this case a spatial repellent, to reduce the risk of ABV transmission compared to a placebo.

Published

2022

11. Molecular Characterization by Multilocus Sequence Typing and Diversity Analysis of Rickettsia asembonensis in Peru.

Author

Loyola S, Torre A, Flores-Mendoza C, Kocher C, Salmon-Mulanovich G, Richards AL, and Leguia M

Subjects

Animals, Cats, DNA, Bacterial genetics, Dogs, Multilocus Sequence Typing veterinary, Peru epidemiology, Phylogeny, Rickettsia genetics

Abstract

Despite several reports worldwide documenting the presence of Rickettsia asembonensis in samples derived from ectoparasites, animals and more recently humans, genomic information of these specimens remains scarce, and when available, is usually limited to small genomic fragments of limited value. We generated complete sequences for two conserved (17-kDa antigen gene and gltA ) and three variable ( sca4 , ompB and ompA ) genes in five R. asembonensis DNA samples detected in cat and dog fleas in Peru. Complete gene sequences were used to conduct multi-locus sequence typing and phylogenetic analyses to assess diversity and infer relationships among strains and other reference sequences. The 17-kDa antigen gene was highly conserved across Rickettsia species. Of the variable genes ompB was the most variable, but this diversity was not captured through phylogenetics alone even when efforts were made to maximize potential diversity in terms of flea species, animal host and location. Through a combination of de novo and reference-based genome assembly we identified a 75 bp insertion in ompA that encodes a 25 aa repetitive motif found in other Rickettsia species, but not present in the original prototype strain from Kenya. R. asembonensis has only recently been shown to be a bona-fide human pathogen. As such, and compounded by a lack of available genomic information, it remains understudied. Our work directly addresses the lack of genomic information available worldwide for the study of these novel Rickettsia species and specifically contributes to our understanding of the diversity and molecular epidemiology of R. asembonensis in Peru.

Published

2022

12. Cues for seizure timing.

Author

Rao VR, G Leguia M, Tcheng TK, and Baud MO

Subjects

Data Analysis, Humans, Sleep Stages physiology, Time Factors, Circadian Rhythm physiology, Cues, Electroencephalography methods, Seizures diagnosis, Seizures physiopathology

Abstract

The cyclical organization of seizures in epilepsy has been described since antiquity. However, historical explanations for seizure cycles-based on celestial, hormonal, and environmental factors-have only recently become testable with the advent of chronic electroencephalography (cEEG) and modern statistical techniques. Here, factors purported over millennia to influence seizure timing are viewed through a contemporary lens. We discuss the emerging concept that seizures are organized over multiple timescales, each involving differential influences of external and endogenous rhythm generators. Leveraging large cEEG datasets and circular statistics appropriate for cyclical phenomena, we present new evidence for circadian (day-night), multidien (multi-day), and circannual (about-yearly) variation in seizure activity. Modulation of seizure timing by multiscale temporal variables has implications for diagnosis and therapy in clinical epilepsy. Uncovering the mechanistic basis for seizure cycles, particularly the factors that govern multidien periodicity, will be a major focus of future work., (© 2020 International League Against Epilepsy.)

Published

2021

13. Minority Gene Expression Profiling: Probing the Genetic Signatures of Pathogenesis Using Ribosome Profiling.

Author

Vila-Sanjurjo A, Juarez D, Loyola S, Torres M, and Leguia M

Subjects

Cell Line, Humans, Sequence Analysis, RNA, Dengue virology, Dengue Virus genetics, Gene Expression Profiling, High-Throughput Nucleotide Sequencing, Ribosomes genetics

Abstract

Minority Gene Expression Profiling (MGEP) refers to a scenario where the expression profiles of specific genes of interest are concentrated in a small cellular pool that is embedded within a larger, non-expressive pool. An example of this is the analysis of disease-related genes within sub-populations of blood or biopsied tissues. These systems are characterized by low signal-to-noise ratios that make it difficult, if not impossible, to uncover the desired signatures of pathogenesis in the absence of lengthy, and often problematic, technical manipulations. We have adapted ribosome profiling (RP) workflows from the Illumina to the Ion Proton platform and used them to analyze signatures of pathogenesis in an MGEP model system consisting of human cells eliciting <3% productive dengue infection. We find that RP is powerful enough to identify relevant responses of differentially expressed genes, even in the presence of significant noise. We discuss how to deal with sources of unwanted variation, and propose ways to further improve this powerful approach to the study of pathogenic signatures within MGEP systems., (© The Author(s) 2020. Published by Oxford University Press for the Infectious Diseases Society of America. All rights reserved. For permissions, e-mail: journals.permissions@oup.com.)

Published

2020

14. Precision Medicine and Precision Public Health in the Era of Pathogen Next-Generation Sequencing.

Author

Leguia M, Vila-Sanjurjo A, Chain PSG, Berry IM, Jarman RG, and Pollett S

Subjects

Communicable Diseases parasitology, Communicable Diseases virology, Humans, Communicable Diseases microbiology, Genomics, High-Throughput Nucleotide Sequencing, Precision Medicine, Public Health

Abstract

This brief report serves as an introduction to a supplement of the Journal of Infectious Diseases entitled "Next-Generation Sequencing (NGS) Technologies to Advance Global Infectious Disease Research." We briefly discuss the history of NGS technologies and describe how the techniques developed during the past 40 years have impacted our understanding of infectious diseases. Our focus is on the application of NGS in the context of pathogen genomics. Beyond obvious clinical and public health applications, we also discuss the challenges that still remain within this rapidly evolving field., (© The Author(s) 2019. Published by Oxford University Press for the Infectious Diseases Society of America. All rights reserved. For permissions, e-mail: journals.permissions@oup.com.)

Published

2020

15. Seroprevalence and Risk Factors for Rickettsia and Leptospira Infection in Four Ecologically Distinct Regions of Peru.

Author

Salmon-Mulanovich G, Simons MP, Flores-Mendoza C, Loyola S, Silva M, Kasper M, Rázuri HR, Canal LE, Leguia M, Bausch DG, and Richards AL

Subjects

Adolescent, Adult, Animals, Animals, Domestic, Antibodies, Bacterial blood, Child, Child, Preschool, Cross-Sectional Studies, Demography, Ecosystem, Ectoparasitic Infestations epidemiology, Ectoparasitic Infestations parasitology, Ectoparasitic Infestations veterinary, Female, Humans, Infant, Infant, Newborn, Leptospira immunology, Leptospirosis microbiology, Male, Middle Aged, Peru epidemiology, Pets, Rickettsia immunology, Rickettsia Infections microbiology, Risk Factors, Seroepidemiologic Studies, Young Adult, Zoonoses, Leptospirosis epidemiology, Rickettsia Infections epidemiology

Abstract

Rickettsia and Leptospira spp. are under-recognized causes of acute febrile disease worldwide. Rickettsia species are often placed into the spotted fever group rickettsiae (SFGR) and typhus group rickettsiae (TGR). We explored the antibody prevalence among humans for these two groups of rickettsiae in four regions of Peru (Lima, Cusco, Puerto Maldonado, and Tumbes) and for Leptospira spp. in Puerto Maldonado and Tumbes. We also assessed risk factors for seropositivity and collected serum samples and ectoparasites from peri-domestic animals from households in sites with high human seroprevalence. In total, we tested 2,165 human sera for antibodies (IgG) against SFGR and TGR by ELISA and for antibodies against Leptospira by a microscopic agglutination test. Overall, human antibody prevalence across the four sites was 10.6% for SFGR (ranging from 6.2% to 14.0%, highest in Tumbes) and 3.3% for TGR (ranging from 2.6% to 6.4%, highest in Puerto Maldonado). Factors associated with seroreactivity against SFGR were male gender, older age, contact with backyard birds, and working in agriculture or with livestock. However, exposure to any kind of animal within the household decreased the odds ratio by half. Age was the only variable associated with higher TGR seroprevalence. The prevalence of Leptospira was 11.3% in Puerto Maldonado and 5.8% in Tumbes, with a borderline association with keeping animals in the household. We tested animal sera for Leptospira and conducted polymerase chain reaction (PCR) to detect Rickettsia species among ectoparasites collected from domestic animals in 63 households of seropositive participants and controls. We did not find any association between animal infection and human serostatus.

Published

2019

16. Isolation of Complete Equine Encephalitis Virus Genome from Human Swab Specimen, Peru.

Author

Juarez D, Guevara C, Wiley M, Torre A, Palacios G, Halsey ES, Ampuero S, and Leguia M

Subjects

Adolescent, Animals, Chlorocebus aethiops, Dogs, Encephalitis Virus, Venezuelan Equine classification, Encephalitis Virus, Venezuelan Equine isolation & purification, Encephalomyelitis, Venezuelan Equine transmission, Encephalomyelitis, Venezuelan Equine virology, Horses, Humans, Madin Darby Canine Kidney Cells, Male, Nasopharynx virology, Peru, Vero Cells, Whole Genome Sequencing, Antibodies, Viral blood, Encephalitis Virus, Venezuelan Equine genetics, Encephalomyelitis, Venezuelan Equine diagnosis, Genome, Viral

Abstract

While studying respiratory infections in Peru, we identified Venezuelan equine encephalitis virus (VEEV) in a nasopharyngeal swab, indicating that this alphavirus can be present in human respiratory secretions. Because VEEV may be infectious when aerosolized, our finding is relevant for the management of VEEV-infected patients and for VEEV transmission studies.

Published

2018

17. The transmission dynamics and diversity of human metapneumovirus in Peru.

Author

Pollett S, Trovão NS, Tan Y, Eden JS, Halpin RA, Bera J, Das SR, Wentworth D, Ocaña V, Mendocilla SM, Álvarez C, Calisto ME, Garcia J, Halsey E, Ampuero JS, Nelson MI, and Leguia M

Subjects

Adolescent, Adult, Aged, Child, Child, Preschool, Female, Genome, Viral, Humans, Infant, Male, Middle Aged, Paramyxoviridae Infections epidemiology, Peru epidemiology, Young Adult, Genetic Variation, Metapneumovirus genetics, Paramyxoviridae Infections transmission, Paramyxoviridae Infections virology

Abstract

Background: The transmission dynamics of human metapneumovirus (HMPV) in tropical countries remain unclear. Further understanding of the genetic diversity of the virus could aid in HMPV vaccine design and improve our understanding of respiratory virus transmission dynamics in low- and middle-income countries., Materials & Methods: We examined the evolution of HMPV in Peru through phylogenetic analysis of 61 full genome HMPV sequences collected in three ecologically diverse regions of Peru (Lima, Piura, and Iquitos) during 2008-2012, comprising the largest data set of HMPV whole genomes sequenced from any tropical country to date., Results: We revealed extensive genetic diversity generated by frequent viral introductions, with little evidence of local persistence. While considerable viral traffic between non-Peruvian countries and Peru was observed, HMPV epidemics in Peruvian locales were more frequently epidemiologically linked with other sites within Peru. We showed that Iquitos experienced greater HMPV traffic than the similar sized city of Piura by both Bayesian and maximum likelihood methods., Conclusions: There is extensive HMPV genetic diversity even within smaller and relatively less connected cities of Peru and this virus is spatially fluid. Greater diversity of HMPV in Iquitos compared to Piura may relate to higher volumes of human movement, including air traffic to this location., (© 2017 The Authors. Influenza and Other Respiratory Viruses Published by John Wiley & Sons Ltd.)

Published

2018

18. Rickettsia asembonensis Characterization by Multilocus Sequence Typing of Complete Genes, Peru.

Author

Loyola S, Flores-Mendoza C, Torre A, Kocher C, Melendrez M, Luce-Fedrow A, Maina AN, Richards AL, and Leguia M

Subjects

Animals, Peru, Phylogeny, Rickettsia classification, Siphonaptera microbiology, DNA, Bacterial genetics, Multilocus Sequence Typing, Rickettsia genetics, Rickettsia isolation & purification

Abstract

While studying rickettsial infections in Peru, we detected Rickettsia asembonensis in fleas from domestic animals. We characterized 5 complete genomic regions (17kDa, gltA, ompA, ompB, and sca4) and conducted multilocus sequence typing and phylogenetic analyses. The molecular isolate from Peru is distinct from the original R. asembonensis strain from Kenya.

Published

2018

19. Full-genome amplification and sequencing of Zika viruses using a targeted amplification approach.

Author

Leguia M, Cruz CD, Felices V, Torre A, Troncos G, Espejo V, Guevara C, and Mores C

Subjects

DNA Primers, DNA, Complementary, High-Throughput Nucleotide Sequencing economics, Humans, Nucleic Acid Amplification Techniques economics, RNA, Viral genetics, Sequence Analysis, DNA methods, Genome, Viral, High-Throughput Nucleotide Sequencing methods, Nucleic Acid Amplification Techniques methods, Polymerase Chain Reaction methods, Zika Virus genetics

Abstract

We have developed methods for full-genome sequencing of Zika viruses (ZIKVs) based on a targeted amplification approach. We used alignments of publicly available complete genome data to design a primer set that selectively amplifies ZIKVs. The approach includes amplification strategies for templates present at both high- and low-copy number, and PCR cycling conditions that have been normalized across genome fragments in order to streamline laboratory handling. Abundant templates can be amplified using a strategy that uses 6 overlapping amplicons to cover the complete viral genome, whereas scarce templates can be amplified using a strategy that uses 11 overlapping amplicons of smaller size. The workflow is sequencing platform agnostic, and thus, can be used in low resource settings where access to traditional Sanger sequencing is the only option available. Given the scarcity of tools for ZIKV, this approach should facilitate epidemiological surveillance and other studies that require the generation of complete viral genomic information quickly and cost-effectively., (Published by Elsevier B.V.)

Published

2017

20. Serologic Evidence of Scrub Typhus in the Peruvian Amazon.

Author

Kocher C, Jiang J, Morrison AC, Castillo R, Leguia M, Loyola S, Ampuero JS, Cespedes M, Halsey ES, Bausch DG, and Richards AL

Subjects

Humans, Peru epidemiology, Population Surveillance, Retrospective Studies, Scrub Typhus immunology, Seroepidemiologic Studies, Scrub Typhus epidemiology

Abstract

Using a large, passive, febrile surveillance program in Iquitos, Peru, we retrospectively tested human blood specimens for scrub typhus group orientiae by ELISA, immunofluorescence assay, and PCR. Of 1,124 participants, 60 (5.3%) were seropositive, and 1 showed evidence of recent active infection. Our serologic data indicate that scrub typhus is present in the Peruvian Amazon.

Published

2017

21. Whole-Genome Analysis of Bartonella ancashensis, a Novel Pathogen Causing Verruga Peruana, Rural Ancash Region, Peru.

Author

Mullins KE, Hang J, Clifford RJ, Onmus-Leone F, Yang Y, Jiang J, Leguia M, Kasper MR, Maguina C, Lesho EP, Jarman RG, Richards A, and Blazes D

Subjects

Adolescent, Adult, Bartonella classification, Bartonella Infections epidemiology, Child, Child, Preschool, Female, Humans, Infant, Male, Middle Aged, Peru epidemiology, Phylogeny, Young Adult, Bartonella genetics, Bartonella Infections microbiology, Genome, Bacterial

Abstract

The genus Bartonella contains >40 species, and an increasing number of these Bartonella species are being implicated in human disease. One such pathogen is Bartonella ancashensis, which was isolated in blood samples from 2 patients living in Caraz, Peru, during a clinical trial of treatment for bartonellosis. Three B. ancashensis strains were analyzed by using whole-genome restriction mapping and high-throughput pyrosequencing. Genome-wide comparative analysis of Bartonella species showed that B. ancashensis has features seen in modern and ancient lineages of Bartonella species and is more related to B. bacilliformis. The divergence between B. ancashensis and B. bacilliformis is much greater than what is seen between known Bartonella genetic lineages. In addition, B. ancashensis contains type IV secretion system proteins, which are not present in B. bacilliformis. Whole-genome analysis indicates that B. ancashensis might represent a distinct Bartonella lineage phylogenetically related to B. bacilliformis.

Published

2017

22. Targeted full-genome amplification and sequencing of dengue virus types 1-4 from South America.

Author

Cruz CD, Torre A, Troncos G, Lambrechts L, and Leguia M

Subjects

DNA Primers, Dengue virology, Dengue Virus isolation & purification, Evolution, Molecular, Genotype, Humans, Polymerase Chain Reaction methods, RNA, Viral genetics, Sequence Analysis, DNA methods, Dengue Virus genetics, Genome, Viral, High-Throughput Nucleotide Sequencing

Abstract

We report optimized workflows for full-genome sequencing of dengue viruses (DENVs) 1-4. Based on alignments of publicly available complete genomes we modified and expanded existing primers sets to amplify DENV genotypes that were previously difficult or impossible to sequence. We also report improvements to streamline laboratory handling, including a dual amplification strategy for easy and difficult to sequence "high-copy" and "low-copy" templates, respectively, and normalization of PCR cycling conditions across serotypes. High-copy templates can be sequenced following amplification of as few as 5 overlapping segments covering the complete viral genome, whereas low-copy templates can be sequenced following amplification of no more than 10 overlapping segments of smaller size. These changes have been validated using a balanced set of wild-type DENV genomes (11 of DENV1, 14 of DENV2, 13 of DENV3 and 7 of DENV4) derived from human serum samples collected throughout South America over the past 15 years. The changes described enable generation of complete DENV genomes from wild-type samples without the need for viral enrichment via passaging through laboratory cell lines. This should facilitate quick and cost-effective generation of DENV full-genome sequences of the type needed for accurate epidemiological surveillance and thorough evolutionary studies of wild-type DENVs., (Published by Elsevier B.V.)

Published

2016

23. Rickettsial Disease in the Peruvian Amazon Basin.

Author

Kocher C, Morrison AC, Leguia M, Loyola S, Castillo RM, Galvez HA, Astete H, Flores-Mendoza C, Ampuero JS, Bausch DG, Halsey ES, Cespedes M, Zevallos K, Jiang J, and Richards AL

Subjects

Adolescent, Adult, Animals, Antibodies, Bacterial blood, Child, Female, Humans, Male, Peru epidemiology, Rickettsia genetics, Rickettsia physiology, Rickettsia Infections blood, Rickettsia Infections epidemiology, Rickettsia Infections transmission, Siphonaptera classification, Siphonaptera microbiology, Young Adult, Rickettsia isolation & purification, Rickettsia Infections microbiology

Abstract

Using a large, passive, clinic-based surveillance program in Iquitos, Peru, we characterized the prevalence of rickettsial infections among undifferentiated febrile cases and obtained evidence of pathogen transmission in potential domestic reservoir contacts and their ectoparasites. Blood specimens from humans and animals were assayed for spotted fever group rickettsiae (SFGR) and typhus group rickettsiae (TGR) by ELISA and/or PCR; ectoparasites were screened by PCR. Logistic regression was used to determine associations between patient history, demographic characteristics of participants and symptoms, clinical findings and outcome of rickettsial infection. Of the 2,054 enrolled participants, almost 2% showed evidence of seroconversion or a 4-fold rise in antibody titers specific for rickettsiae between acute and convalescent blood samples. Of 190 fleas (Ctenocephalides felis) and 60 ticks (Rhipicephalus sanguineus) tested, 185 (97.4%) and 3 (5%), respectively, were positive for Rickettsia spp. Candidatus Rickettsia asemboensis was identified in 100% and 33% of the fleas and ticks tested, respectively. Collectively, our serologic data indicates that human pathogenic SFGR are present in the Peruvian Amazon and pose a significant risk of infection to individuals exposed to wild, domestic and peri-domestic animals and their ectoparasites.

Published

2016

24. Full Genomic Characterization of a Saffold Virus Isolated in Peru.

Author

Leguia M, Loyola S, Rios J, Juarez D, Guevara C, Silva M, Prieto K, Wiley M, Kasper MR, Palacios G, and Bausch DG

Abstract

While studying respiratory infections of unknown etiology we detected Saffold virus in an oropharyngeal swab collected from a two-year-old female suffering from diarrhea and respiratory illness. The full viral genome recovered by deep sequencing showed 98% identity to a previously described Saffold strain isolated in Japan. Phylogenetic analysis confirmed the Peruvian Saffold strain belongs to genotype 3 and is most closely related to strains that have circulated in Asia. This is the first documented case report of Saffold virus in Peru and the only complete genomic characterization of a Saffold-3 isolate from the Americas.

Published

2015

25. Complete Genome Sequence of Bartonella ancashensis Strain 20.00, Isolated from the Blood of a Patient with Verruga Peruana.

Author

Hang J, Mullins KE, Clifford RJ, Onmus-Leone F, Yang Y, Jiang J, Leguia M, Kasper MR, Maguiña C, Lesho EP, Jarman RG, Richards AL, and Blazes D

Abstract

Here we present the complete genome sequence of Bartonella ancashensis strain 20.00, isolated from the blood of a Peruvian patient with verruga peruana, known as Carrion's disease. Bartonella ancashensis is a Gram-negative bacillus, phylogenetically most similar to Bartonella bacilliformis, the causative agent of Oroya fever and verruga peruana., (Copyright © 2015 Hang et al.)

Published

2015

26. Description of Bartonella ancashensis sp. nov., isolated from the blood of two patients with verruga peruana.

Author

Mullins KE, Hang J, Jiang J, Leguia M, Kasper MR, Ventosilla P, Maguiña C, Jarman RG, Blazes D, and Richards AL

Subjects

Bacterial Typing Techniques, Bartonella genetics, Bartonella isolation & purification, Bartonella Infections blood, Base Composition, Child, Child, Preschool, DNA, Bacterial genetics, DNA, Ribosomal Spacer genetics, Fatty Acids chemistry, Genes, Bacterial, Genotype, Humans, Male, Molecular Sequence Data, Peru, RNA, Ribosomal, 16S genetics, RNA, Ribosomal, 23S genetics, Sequence Analysis, DNA, Bartonella classification, Bartonella Infections microbiology, Phylogeny

Abstract

Three novel isolates of the genus Bartonella were recovered from the blood of two patients enrolled in a clinical trial for the treatment of chronic stage Bartonella bacilliformis infection (verruga peruana) in Caraz, Ancash, Peru. The isolates were initially characterized by sequencing a fragment of the gltA gene, and found to be disparate from B. bacilliformis. The isolates were further characterized using phenotypic and genotypic methods, and found to be genetically identical to each other for the genes assessed, but distinct from any known species of the genus Bartonella, including the closest relative B. bacilliformis. Other characteristics of the isolates, including their morphology, microscopic and biochemical properties, and growth patterns, were consistent with members of the genus Bartonella. Based on these results, we conclude that these three isolates are members of a novel species of the genus Bartonella for which we propose the name Bartonella ancashensis sp. nov. (type strain 20.00T = ATCC BAA-2694T = DSM 29364T).

Published

2015

27. Molecular typing of "Candidatus Bartonella ancashi," a new human pathogen causing verruga peruana.

Author

Mullins KE, Hang J, Jiang J, Leguia M, Kasper MR, Maguiña C, Jarman RG, Blazes DL, and Richards AL

Subjects

Animals, Bartonella isolation & purification, Bartonella bacilliformis, Child, Preschool, Cluster Analysis, DNA, Bacterial chemistry, DNA, Bacterial genetics, Humans, Male, Molecular Sequence Data, Peru, Phylogeny, Sequence Analysis, DNA, Sequence Homology, Bartonella classification, Bartonella genetics, Bartonella Infections microbiology, Molecular Typing methods

Abstract

A recently described clinical isolate, "Candidatus Bartonella ancashi," was obtained from a blood sample of a patient presenting with verruga peruana in the Ancash region of Peru. This sample and a second isolate obtained 60 days later from the same patient were molecularly typed using multilocus sequence typing (MLST) and multispacer sequence typing (MST). The isolates were 100% indistinguishable from each other but phylogenetically distant from Bartonella bacilliformis and considerably divergent from other known Bartonella species, confirming their novelty.

Published

2013

28. Molecular epidemiology of American/Asian genotype DENV-2 in Peru.

Author

Cruz CD, Forshey BM, Juarez DS, Guevara C, Leguia M, Kochel TJ, and Halsey ES

Subjects

Dengue transmission, Dengue Virus classification, Genotype, Humans, Molecular Epidemiology, Peru epidemiology, Phylogeny, Phylogeography, RNA, Viral analysis, Dengue epidemiology, Dengue virology, Dengue Virus genetics

Abstract

During the past decade, countries in South America have reported dengue hemorrhagic fever (DHF) associated with American/Asian genotype of dengue virus serotype 2 (DENV-2). DENV-2 strains have been associated with large outbreaks of dengue fever and DHF in numerous regions of Peru since the mid-1990s, but studies to address the origins, distribution, and genetic diversity of DENV-2 strains have been limited. To address this knowledge gap, we sequenced the envelope gene region of DENV-2 isolates from Peru, Ecuador, Paraguay, and Bolivia. Sequences were aligned and compared to a global sample of DENV-2 viruses. Phylogenetic analysis confirmed the circulation of two DENV-2 genotypes in Peru: American (prior to 2001) and American/Asian (2000 to present). American/Asian genotype variants can be classified into two lineages, and these were introduced into Peru from the north (Ecuador, Colombia, and/or Venezuela) and the east (Brazil and Bolivia). American/Asian lineage II replaced lineage I after 2009. We estimate the time to the most recent common ancestor for American/Asian DENV-2 genotype in the Americas was in 1980, and 1984 and 1989 for lineages I and II, respectively. In light of evidence for increased virulence of lineage II of American/Asian DENV-2, our results support the need for continuous monitoring for the emergence of new DENV genotypes that may be associated with severe disease., (Copyright © 2013. Published by Elsevier B.V.)

Published

2013

29. Genomic analysis of two novel human enterovirus C genotypes found in respiratory samples from Peru.

Author

Tokarz R, Hirschberg DL, Sameroff S, Haq S, Luna G, Bennett AJ, Silva M, Leguia M, Kasper M, Bausch DG, and Lipkin WI

Subjects

5' Untranslated Regions, Amino Acid Sequence, Base Sequence, Cohort Studies, Genomics methods, Genotype, Humans, Molecular Sequence Data, Peru, Phylogeny, Viral Nonstructural Proteins, Enterovirus C, Human genetics, Enterovirus Infections virology, Genome, Viral, Respiratory System virology, Respiratory Tract Diseases virology

Abstract

We report the discovery of two enteroviruses detected in nasopharyngeal samples obtained from subjects with respiratory disease in Peru. Phylogenetic analysis indicated that both viruses belong to a clade within the species Human enterovirus C, which includes the recently characterized human enteroviruses 109 and 104. Members of this clade have undergone significant genomic rearrangement, as indicated by deletions in the hypervariable region of the 5' UTR and the VP1 protein, as well as recombination within the non-structural genes. Our findings and review of published sequences suggests that several novel human enterovirus C serotypes are currently circulating worldwide.

Published

2013

30. Histamine is a modulator of metamorphic competence in Strongylocentrotus purpuratus (Echinodermata: Echinoidea).

Author

Sutherby J, Giardini JL, Nguyen J, Wessel G, Leguia M, and Heyland A

Subjects

Animals, Apoptosis, Chlorpheniramine pharmacology, Cimetidine pharmacology, Ectoderm cytology, Gene Expression Regulation, Developmental, Histamine metabolism, Histamine H1 Antagonists pharmacology, Histamine H2 Antagonists pharmacology, Histamine H3 Antagonists pharmacology, Histidine Decarboxylase antagonists & inhibitors, Larva cytology, Larva drug effects, Larva growth & development, Larva metabolism, Metamorphosis, Biological, Methylhistidines pharmacology, Organ Specificity, Piperidines pharmacology, Receptors, Histamine H1 genetics, Receptors, Histamine H1 metabolism, Strongylocentrotus purpuratus cytology, Strongylocentrotus purpuratus drug effects, Strongylocentrotus purpuratus metabolism, Histamine physiology, Strongylocentrotus purpuratus growth & development

Abstract

Background: A metamorphic life-history is present in the majority of animal phyla. This developmental mode is particularly prominent among marine invertebrates with a bentho-planktonic life cycle, where a pelagic larval form transforms into a benthic adult. Metamorphic competence (the stage at which a larva is capable to undergo the metamorphic transformation and settlement) is an important adaptation both ecologically and physiologically. The competence period maintains the larval state until suitable settlement sites are encountered, at which point the larvae settle in response to settlement cues. The mechanistic basis for metamorphosis (the morphogenetic transition from a larva to a juvenile including settlement), i.e. the molecular and cellular processes underlying metamorphosis in marine invertebrate species, is poorly understood. Histamine (HA), a neurotransmitter used for various physiological and developmental functions among animals, has a critical role in sea urchin fertilization and in the induction of metamorphosis. Here we test the premise that HA functions as a developmental modulator of metamorphic competence in the sea urchin Strongylocentrotus purpuratus., Results: Our results provide strong evidence that HA leads to the acquisition of metamorphic competence in S. purpuratus larvae. Pharmacological analysis of several HA receptor antagonists and an inhibitor of HA synthesis indicates a function of HA in metamorphic competence as well as programmed cell death (PCD) during arm retraction. Furthermore we identified an extensive network of histaminergic neurons in pre-metamorphic and metamorphically competent larvae. Analysis of this network throughout larval development indicates that the maturation of specific neuronal clusters correlates with the acquisition of metamorphic competence. Moreover, histamine receptor antagonist treatment leads to the induction of caspase mediated apoptosis in competent larvae., Conclusions: We conclude that HA is a modulator of metamorphic competence in S. purpuratus development and hypothesize that HA may have played an important role in the evolution of settlement strategies in echinoids. Our findings provide novel insights into the evolution of HA signalling and its function in one of the most important and widespread life history transitions in the animal kingdom--metamorphosis.

Published

2012

31. Eugene--a domain specific language for specifying and constraining synthetic biological parts, devices, and systems.

Author

Bilitchenko L, Liu A, Cheung S, Weeding E, Xia B, Leguia M, Anderson JC, and Densmore D

Subjects

Algorithms, Automation, Computational Biology methods, Computer Simulation, DNA genetics, Humans, Software, Biology methods, Language, Synthetic Biology methods

Abstract

Background: Synthetic biological systems are currently created by an ad-hoc, iterative process of specification, design, and assembly. These systems would greatly benefit from a more formalized and rigorous specification of the desired system components as well as constraints on their composition. Therefore, the creation of robust and efficient design flows and tools is imperative. We present a human readable language (Eugene) that allows for the specification of synthetic biological designs based on biological parts, as well as provides a very expressive constraint system to drive the automatic creation of composite Parts (Devices) from a collection of individual Parts., Results: We illustrate Eugene's capabilities in three different areas: Device specification, design space exploration, and assembly and simulation integration. These results highlight Eugene's ability to create combinatorial design spaces and prune these spaces for simulation or physical assembly. Eugene creates functional designs quickly and cost-effectively., Conclusions: Eugene is intended for forward engineering of DNA-based devices, and through its data types and execution semantics, reflects the desired abstraction hierarchy in synthetic biology. Eugene provides a powerful constraint system which can be used to drive the creation of new devices at runtime. It accomplishes all of this while being part of a larger tool chain which includes support for design, simulation, and physical device assembly.

Published

2011

32. Automated assembly of standard biological parts.

Author

Leguia M, Brophy J, Densmore D, and Anderson JC

Subjects

Base Sequence, High-Throughput Screening Assays, Plasmids genetics, Robotics, User-Computer Interface, Automation methods, DNA chemical synthesis, Software, Synthetic Biology methods

Abstract

The primary bottleneck in synthetic biology research today is the construction of physical DNAs, a process that is often expensive, time-consuming, and riddled with cloning difficulties associated with the uniqueness of each DNA sequence. We have developed a series of biological and computational tools that lower existing barriers to automation and scaling to enable affordable, fast, and accurate construction of large DNA sets. Here we provide detailed protocols for high-throughput, automated assembly of BglBrick standard biological parts using iterative 2ab reactions. We have implemented these protocols on a minimal hardware platform consisting of a Biomek 3000 liquid handling robot, a benchtop centrifuge and a plate thermocycler, with additional support from a software tool called AssemblyManager. This methodology enables parallel assembly of several hundred large error-free DNAs with a 96+% success rate., (Copyright © 2011 Elsevier Inc. All rights reserved.)

Published

2011

33. BglBricks: A flexible standard for biological part assembly.

Author

Anderson JC, Dueber JE, Leguia M, Wu GC, Goler JA, Arkin AP, and Keasling JD

Abstract

Background: Standard biological parts, such as BioBricks parts, provide the foundation for a new engineering discipline that enables the design and construction of synthetic biological systems with a variety of applications in bioenergy, new materials, therapeutics, and environmental remediation. Although the original BioBricks assembly standard has found widespread use, it has several shortcomings that limit its range of potential applications. In particular, the system is not suitable for the construction of protein fusions due to an unfavorable scar sequence that encodes an in-frame stop codon., Results: Here, we present a similar but new composition standard, called BglBricks, that addresses the scar translation issue associated with the original standard. The new system employs BglII and BamHI restriction enzymes, robust cutters with an extensive history of use, and results in a 6-nucleotide scar sequence encoding glycine-serine, an innocuous peptide linker in most protein fusion applications. We demonstrate the utility of the new standard in three distinct applications, including the construction of constitutively active gene expression devices with a wide range of expression profiles, the construction of chimeric, multi-domain protein fusions, and the targeted integration of functional DNA sequences into specific loci of the E. coli genome., Conclusions: The BglBrick standard provides a new, more flexible platform from which to generate standard biological parts and automate DNA assembly. Work on BglBrick assembly reactions, as well as on the development of automation and bioinformatics tools, is currently underway. These tools will provide a foundation from which to transform genetic engineering from a technically intensive art into a purely design-based discipline.

Published

2010

34. The histamine H1 receptor activates the nitric oxide pathway at fertilization.

Author

Leguia M and Wessel GM

Subjects

Amino Acid Sequence, Animals, Antigens, Surface metabolism, Models, Biological, Molecular Sequence Data, Nitric Oxide biosynthesis, Ovum metabolism, Receptors, Histamine H1 metabolism, Sea Urchins metabolism, Sea Urchins physiology, Sequence Homology, Amino Acid, Signal Transduction, Fertilization physiology, Nitric Oxide metabolism, Receptors, Histamine H1 physiology

Abstract

Sperm fusion with the egg initiates a signaling cascade that releases intracellular calcium (Ca(i) (2+)) from the endoplasmic reticulum (ER). In sea urchins, Ca(2+) is released as a single, large transient via two distinct pathways. The first depends on inositol 1,4,5-triphosphate (IP(3)) production and triggers the initial phase of Ca(2+) release, while the second depends on nitric oxide (NO) production and is thought to maintain the duration of the Ca(2+) wave. We identified a sea urchin homolog of the seven trans-membrane G protein-coupled receptor for histamine (suH(1)R) on the egg cell surface that activates NO production. Treatment with histamine (HA) causes fluctuations in the resting levels of NO in the egg, while antagonists or antibodies of H(1)R inhibit the rise of NO normally observed at fertilization. Inhibition of suH(1)R function decreases the maintenance, but not the amplitude, of the Ca(2+) transient and suggests that it is an integral part of the overall pathway leading to egg activation at fertilization in sea urchins.

Published

2006

35. Synaptotagmin I is involved in the regulation of cortical granule exocytosis in the sea urchin.

Author

Leguia M, Conner S, Berg L, and Wessel GM

Subjects

Animals, DNA, Complementary genetics, Gene Expression Regulation, Developmental, Ovum cytology, Sea Urchins genetics, Sequence Alignment, Synaptotagmins chemistry, Synaptotagmins genetics, Exocytosis, Fertilization, Ovum physiology, Sea Urchins physiology, Secretory Vesicles physiology, Synaptotagmins physiology

Abstract

Cortical granules are stimulus-dependent secretory vesicles found in the egg cortex of most vertebrates and many invertebrates. Upon fertilization, an increase in intracellular calcium levels triggers cortical granules to exocytose enzymes and structural proteins that permanently modify the extracellular surface of the egg to prevent polyspermy. Synaptotagmin is postulated to be a calcium sensor important for stimulus-dependent secretion and to test this hypothesis for cortical granule exocytosis, we identified the ortholog in two sea urchin species that is present selectively on cortical granules. Characterization by RT-PCR, in-situ RNA hybridization, Western blot and immunolocalization shows that synaptotagmin I is expressed in a manner consistent with it having a role during cortical granule secretion. We specifically tested synaptotagmin function during cortical granule exocytosis using a microinjected antibody raised against the entire cytoplasmic domain of sea urchin synaptotagmin I. The results show that synaptotagmin I is essential for normal cortical granule dynamics at fertilization in the sea urchin egg. Identification of this same protein in other developmental stages also shown here will be important for interpreting stimulus-dependent secretory events for signaling throughout embryogenesis.

Published

2006

36. Selective expression of a sec1/munc18 member in sea urchin eggs and embryos.

Author

Leguia M and Wessel GM

Subjects

Amino Acid Sequence, Animals, Binding, Competitive, Cell Membrane metabolism, Electrophoresis, Exocytosis, Humans, Immunoblotting, Lytechinus, Membrane Proteins biosynthesis, Membrane Proteins metabolism, Microscopy, Fluorescence, Molecular Sequence Data, Munc18 Proteins, Phylogeny, Qa-SNARE Proteins, Reverse Transcriptase Polymerase Chain Reaction, Sea Urchins, Sequence Analysis, DNA, Sequence Homology, Amino Acid, Species Specificity, Strongylocentrotus purpuratus, Synaptosomal-Associated Protein 25, Time Factors, Tissue Distribution, Vesicular Transport Proteins chemistry, Gene Expression Regulation, Developmental, Nerve Tissue Proteins biosynthesis, Vesicular Transport Proteins biosynthesis

Abstract

Regulated secretion is mediated by SNAREs (soluble NSF attachment receptors) and their regulators and effectors, which include the SM (sec1/munc18) family of proteins. Homologs of the SNAREs have been identified in sea urchins, associated with cortical granule exocytosis at fertilization, with membranes of the cleavage furrow, and in secretory cells later in development. To contribute to the understanding of regulated secretion in sea urchins we have cloned the single SM protein homolog from two species of sea urchin, Lytechinus variegatus and Strongylocentrotus purpuratus. In oocytes and eggs, we find that it localizes to the plasma membrane and the cortical region of the egg, consistent with a role in one of the steps leading to cortical granule exocytosis. The protein is also expressed throughout development, enriched in membranes of the cleavage furrow in early embryos, and in cells of the gut in advanced embryos. Furthermore, we find that sec1/munc18 co-localizes with its cognate binding partner syntaxin. Finally, our biochemical analysis shows that the protein associates with rab3 in high molecular weight complexes, suggesting that the exocytotic machinery functions as a multi-protein subunit to mediate regulated secretion in sea urchins. These results will be instrumental in the future to functionally test the SNARE regulators associated with multiple membrane fusion events.

Published

2004

37. Ku86 autoantigen related protein-1 transcription initiates from a CpG island and is induced by p53 through a nearby p53 response element.

Author

Braastad CD, Leguia M, and Hendrickson EA

Subjects

5' Flanking Region, Base Sequence, Carrier Proteins biosynthesis, DNA Methylation, Deoxyribonuclease I chemistry, Fatty Acid Desaturases biosynthesis, Fatty Acid Desaturases genetics, Humans, Ku Autoantigen, Molecular Sequence Data, Oxidoreductases Acting on CH-CH Group Donors, RNA, Messenger biosynthesis, Radiation, Ionizing, Transcription Initiation Site, Tumor Cells, Cultured, Carrier Proteins genetics, CpG Islands, DNA Helicases, NADH, NADPH Oxidoreductases, Response Elements, Transcriptional Activation, Tumor Suppressor Protein p53 metabolism

Abstract

The human Ku86 gene and an isoform, KARP-1 (Ku86 autoantigen related protein-1), encode overlapping, but differentially regulated, transcripts. Ku86 is constitutively transcribed at high levels and, although it plays a seminal role in DNA double-strand break repair, its expression is not induced by DNA damage. KARP-1, in contrast, is expressed constitutively only at low levels and its expression is induced by DNA damage in a p53-dependent fashion. The regulatory elements promoting KARP-1 gene expression and p53 responsiveness, however, were unknown. Here, we report that a strong DNase I hypersensitive site (DHS) resides approximately 25 kb upstream from the Ku86 promoter. This DHS is encompassed by a hypomethylated CpG island. Reporter assays demonstrated that this region corresponded to a promoter(s), which promoted transcription of peroxisomal trans-2-enoyl CoA reductase in the centromeric direction and KARP-1 in the telomeric direction. KARP-1 primer extension products were mapped to this CpG island in the correct transcriptional orientation confirming that KARP-1 transcription initiates from this site. Moreover, a p53 response element within the first intron of the KARP-1 transcriptional unit was identified using chromatin immunoprecipitation and antibodies specific to activated forms of p53. These data expand our understanding of this important DNA repair locus.

Published

2002