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1. CD36 promotes vasculogenic mimicry in melanoma by mediating adhesion to the extracellular matrix

Author

Carmela Martini, Mark DeNichilo, Danielle P. King, Michaelia P. Cockshell, Brenton Ebert, Brian Dale, Lisa M. Ebert, Anthony Woods, and Claudine S. Bonder

Subjects
CD36, Vasculogenic mimicry, Melanoma, Tumor microenvironment, Thrombospondin, Laminin, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282
Abstract

Abstract Background The formation of blood vessels within solid tumors directly contributes to cancer growth and metastasis. Until recently, tumor vasculature was thought to occur exclusively via endothelial cell (EC) lined structures (i.e. angiogenesis), but a second source of tumor vasculature arises from the cancer cells themselves, a process known as vasculogenic mimicry (VM). While it is generally understood that the function of VM vessels is the same as that of EC-lined vessels (i.e. to supply oxygen and nutrients to the proliferating cancer cells), the molecular mechanisms underpinning VM are yet to be fully elucidated. Methods Human VM-competent melanoma cell lines were examined for their VM potential using the in vitro angiogenesis assays (Matrigel), together with inhibition studies using small interfering RNA and blocking monoclonal antibodies. Invasion assays and adhesion assays were used to examine cancer cell function. Results Herein we demonstrate that CD36, a cell surface glycoprotein known to promote angiogenesis by ECs, also supports VM formation by human melanoma cancer cells. In silico analysis of CD36 expression within the melanoma cohort of The Cancer Genome Atlas suggests that melanoma patients with high expression of CD36 have a poorer clinical outcome. Using in vitro ‘angiogenesis’ assays and CD36-knockdown approaches, we reveal that CD36 supports VM formation by human melanoma cells as well as adhesion to, and invasion through, a cancer derived extracellular matrix substrate. Interestingly, thrombospondin-1 (TSP-1), a ligand for CD36 on ECs that inhibits angiogenesis, has no effect on VM formation. Further investigation revealed a role for laminin, but not collagen or fibronectin, as ligands for CD36 expressing melanoma cells. Conclusions Taken together, this study suggests that CD36 is a novel regulator of VM by melanoma cancer cells that is facilitated, at least in part, via integrin-α3 and laminin. Unlike angiogenesis, VM is not perturbed by the presence of TSP-1, thus providing new information on differences between these two processes of tumor vascularization which may be exploited to combat cancer progression.

Published
2021
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2. Male Germ Cell Telomeres and Chemical Pollutants

Author

Gabriella Chieffi Baccari, Giuseppe Iurato, Alessandra Santillo, and Brian Dale

Subjects
telomere, male germ cells, sperm, pollutants, fertility, reproduction, Microbiology, QR1-502
Abstract

In recent decades, male infertility has been correlated with the shortening of sperm telomeres. Telomeres regulate the reproductive lifespan by mediating the synapsis and homologous recombination of chromosomes during gametogenesis. They are composed of thousands of hexanucleotide DNA repeats (TTAGGG) that are coupled to specialized shelterin complex proteins and non-coding RNAs. Telomerase activity in male germ cells ensures that the telomere length is maintained at maximum levels during spermatogenesis, despite telomere shortening due to DNA replication or other genotoxic factors such as environmental pollutants. An emerging body of evidence has associated an exposure to pollutants with male infertility. Although telomeric DNA may be one of the important targets of environmental pollutants, only a few authors have considered it as a conventional parameter for sperm function. The aim of this review is to provide comprehensive and up-to-date data on the research carried out so far on the structure/function of telomeres in spermatogenesis and the influence of environmental pollutants on their functionality. The link between pollutant-induced oxidative stress and telomere length in germ cells is discussed.

Published
2023
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3. A Requirement for ZAK Kinase Activity in Canonical TGF-β Signaling

Author

Shyam Nyati, Areeb Chator, Katerina Schinske, Brandon S Gregg, Brian Dale Ross, and Alnawaz Rehemtulla

Subjects
Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282
Abstract

The sterile alpha motif and leucine zipper containing kinase ZAK (AZK, MLT, MLK7), is a MAPK-kinase kinase (MKKK). Like most MAPKKKs which are known to activate the c-Jun. amino-terminal kinase (JNK) pathway, ZAK has been shown to participate in the transduction of Transforming growth factor-β (TGF-β)-mediated non-canonical signaling. A role for ZAK in SMAD-dependent, canonical TGF-β signaling has not been previously appreciated. Using a combination of functional genomics and biochemical techniques, we demonstrate that ZAK regulates canonical TGFβRI/II signaling in lung and breast cancer cell lines and may serve as a key node in the regulation of TGFBR kinase activity. Remarkably, we demonstrate that siRNA mediated depletion of ZAK strongly inhibited TGF-β dependent SMAD2/3 activation and subsequent promoter activation (SMAD binding element driven luciferase expression; SBE4-Luc). A ZAK specific inhibitor (DHP-2), dose-dependently activated the bioluminescent TGFBR-kinase activity reporter (BTR), blocked TGF-β induced SMAD2/3 phosphorylation and SBE4-Luc activation and cancer cell-invasion. In aggregate, these findings identify a novel role for the ZAK kinase in canonical TGF-β signaling and an invasive cancer cell phenotype thus providing a novel target for TGF-β inhibition.

Published
2016
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11. Data from Molecular Imaging of TGFβ-Induced Smad2/3 Phosphorylation Reveals a Role for Receptor Tyrosine Kinases in Modulating TGFβ Signaling

Author

Alnawaz Rehemtulla, Brian Dale Ross, Mukesh Nyati, Dipankar Ray, Katrina Schinske, and Shyam Nyati

Abstract

Purpose: The dual modality of TGFβ, both as a potent tumor suppressor and a stimulator of tumor progression, invasion, and metastasis, make it a critical target for therapeutic intervention in human cancers. The ability to carry out real-time, noninvasive imaging of TGFβ-activated Smad signaling in live cells and animal models would significantly improve our understanding of the regulation of this unique signaling cascade. To advance these efforts, we developed a highly sensitive molecular imaging tool that repetitively, noninvasively, and dynamically reports on TGFBR1 kinase activity.Experimental Design: The bioluminescent TGFβR1 reporter construct was developed using a split firefly luciferase gene containing a functional sensor of Smad2 phosphorylation, wherein inhibition of TGFβ receptor1 kinase activity leads to an increase in reporter signaling. The reporter was stably transfected into mammalian cells and used to image in vivo and in vitro bioluminescent activity as a surrogate for monitoring TGFBR1 kinase activity.Results: The reporter was successfully used to monitor direct and indirect inhibition of TGFβ-induced Smad2 and SMAD3 phosphorylation in live cells and tumor xenografts and adapted for high-throughput screening, to identify a role for receptor tyrosine kinase inhibitors as modulators of TGFβ signaling.Conclusion: The reporter is a dynamic, noninvasive imaging modality for monitoring TGFβ-induced Smad2 signaling in live cells and tumor xenografts. It has immense potential for identifying novel effectors of R-Smad phosphorylation, for validating drug–target interaction, and for studying TGFβ signaling in different metastasis models. Clin Cancer Res; 17(23); 7424–39. ©2011 AACR.

Published
2023
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17. Undersampling artifact reduction for free-breathing 3D stack-of-radial MRI based on a deep adversarial learning network

Author

Chang Gao, Vahid Ghodrati, Shu-Fu Shih, Holden H. Wu, Yongkai Liu, Marcel Dominik Nickel, Thomas Vahle, Brian Dale, Victor Sai, Ely Felker, Chuthaporn Surawech, Qi Miao, J. Paul Finn, Xiaodong Zhong, and Peng Hu

Subjects
Motion, Respiration, Biomedical Engineering, Biophysics, Image Processing, Computer-Assisted, Radiology, Nuclear Medicine and imaging, Artifacts, Magnetic Resonance Imaging
Abstract

Stack-of-radial MRI allows free-breathing abdominal scans, however, it requires relatively long acquisition time. Undersampling reduces scan time but can cause streaking artifacts and degrade image quality. This study developed deep learning networks with adversarial loss and evaluated the performance of reducing streaking artifacts and preserving perceptual image sharpness.A 3D generative adversarial network (GAN) was developed for reducing streaking artifacts in stack-of-radial abdominal scans. Training and validation datasets were self-gated to 5 respiratory states to reduce motion artifacts and to effectively augment the data. The network used a combination of three loss functions to constrain the anatomy and preserve image quality: adversarial loss, mean-squared-error loss and structural similarity index loss. The performance of the network was investigated for 3-5 times undersampled data from 2 institutions. The performance of the GAN for 5 times accelerated images was compared with a 3D U-Net and evaluated using quantitative NMSE, SSIM and region of interest (ROI) measurements as well as qualitative scores of radiologists.The 3D GAN showed similar NMSE (0.0657 vs. 0.0559, p = 0.5217) and significantly higher SSIM (0.841 vs. 0.798, p 0.0001) compared to U-Net. ROI analysis showed GAN removed streaks in both the background air and the tissue and was not significantly different from the reference mean and variations. Radiologists' scores showed GAN had a significant improvement of 1.6 point (p = 0.004) on a 4-point scale in streaking score while no significant difference in sharpness score compared to the input.3D GAN removes streaking artifacts and preserves perceptual image details.

Published
2022

18. Comparison of sperm preparation methods to improve the recovery of mature spermatozoa in sub-fertile males

Author

Chiara Fasano, Giuseppe D’Andolfi, Loredana Di Matteo, Claudia Forte, Brian Dale, and Elisabetta Tosti

Subjects
Male, Aniline Compounds, Semen, Sperm Motility, Humans, Cell Biology, Spermatozoa, Chromatin, Infertility, Male, Developmental Biology
Abstract

SummaryThe integrity of chromatin in the spermatozoon is essential for reproductive outcome. The aim of this study was to evaluate the most effective and cost-effective method to reduce the percentage of spermatozoa with defects in chromatin decondensation for use in assisted reproductive technologies (ART) procedures. Sperm samples from 15 sub-fertile males were examined at CFA Naples to determine the sperm decondensation index (SDI), using the aniline blue test, before and after preparation, comparing density gradients with two different swim-up approaches. All three techniques led to a reduction in decondensed spermatozoa with no statistical difference (P > 0.05) between the control and the treated sperm. In contrast, we found a highly significant decrease in SDI (P < 0.01) after the two swim-up methods in all the samples, confirming the efficacy of these methods in lowering the percentage of chromatin compaction damage. There was no statistical difference between the two swim-up methods, however swim-up from the pellet led to improved count, motility and the percentage of normal condensed spermatozoa. We suggest that swim-up from the pellet be used in ART on sub-fertile males, both to reduce cell stress by multiple centrifugation and improve the recovery rate of mature spermatozoa.

Published
2022

19. MTHFR (methylenetetrahydrofolate reductase: EC 1.5.1.20) SNPs (single-nucleotide polymorphisms) and homocysteine in patients referred for investigation of fertility

Author

Patrice Clement, Laetitia Jacquesson-Fournols, Michel Brack, Geraldine Viot, Marc Cohen, Silvia Alvarez, Yves Menezo, Brian Dale, Dominique Cornet, Pasquale Patrizio, Arthur Clement, Pierre Mares, Jean Clement Sage, To Minh Huong, Edouard J. Servy, Charles Brami, Guiseppe D' Amato, Edouard Amar, Jacques Chouteau, and Paul Neveux

Subjects
Male, Infertility, Heterozygote, Gender prevalence, Genotype, Homocysteine, Gametes, media_common.quotation_subject, Population, Physiology, Fertility, Single-nucleotide polymorphism, Compound heterozygosity, Polymorphism, Single Nucleotide, Recurrent miscarriages, chemistry.chemical_compound, Genetics, Humans, Medicine, SNP, Genetic Predisposition to Disease, education, MTHFR SNPs, Methylenetetrahydrofolate Reductase (NADPH2), Genetics (clinical), Retrospective Studies, media_common, education.field_of_study, DNA methylation, biology, business.industry, Homozygote, Obstetrics and Gynecology, General Medicine, medicine.disease, digestive system diseases, Abortion, Spontaneous, Reproductive Medicine, chemistry, Methylenetetrahydrofolate reductase, biology.protein, Female, France, business, Developmental Biology
Abstract

Purpose MTHFR, one of the major enzymes in the folate cycle, is known to acquire single-nucleotide polymorphisms that significantly reduce its activity, resulting in an increase in circulating homocysteine. Methylation processes are of crucial importance in gametogenesis, involved in the regulation of imprinting and epigenetic tags on DNA and histones. We have retrospectively assessed the prevalence of MTHFR SNPs in a population consulting for infertility according to gender and studied the impact of the mutations on circulating homocysteine levels. Methods More than 2900 patients having suffered at least two miscarriages (2 to 9) or two failed IVF/ICSI (2 to 10) attempts were included for analysis of MTHFR SNPs C677T and A1298C. Serum homocysteine levels were measured simultaneously. Results We observed no difference in the prevalence of different genetic backgrounds between men and women; only 15% of the patients were found to be wild type. More than 40% of the patients are either homozygous for one SNP or compound heterozygous carriers. As expected, the C677T SNP shows the greatest adverse effect on homocysteine accumulation. The impact of MTHFR SNPs on circulating homocysteine is different in men than in women. Conclusions Determination of MTHFR SNPs in both men and women must be seriously advocated in the presence of long-standing infertility; male gametes, from MTHFR SNPs carriers, are not exempted from exerting a hazardous impact on fertility. Patients should be informed of the pleiotropic medical implications of these SNPs for their own health, as well as for the health of future children.

Published
2021
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20. Can sperm quality influence embryo development and its ploidy? Analysis of 811 blastocysts obtained from different sperm sources

Author

Romualdo Polese, Filomena Scarselli, Brian Dale, Maria Giulia Minasi, and Ermanno Greco

Subjects
Male, Pregnancy Rate, Embryonic Development, Cell Biology, Oligospermia, Aneuploidy, Spermatozoa, Semen Analysis, Blastocyst, Pregnancy, Semen, Humans, Female, Developmental Biology, Azoospermia, Retrospective Studies
Abstract

SummaryThe aim of our study was to evaluate the correlation between sperm quality and ploidy status of the derived blastocysts. We performed a retrospective analysis on a restricted pool of patients enrolling only those who had no female factors. Male patients with genetic factors affecting spermatogenesis were also excluded. We chose a maternal age ≤38 years to decrease the female factor, therefore the male factor was the main component of sterility. We divided the patients in four groups based on semen quality and comparing fertilization, pregnancy and euploidy rates above all. In total, 201 intracytoplasmic sperm injection (ICSI) cycles were enrolled in the study. Cycles were divided into four groups, according to semen source: normal semen, oligoasthenoteratozoospermia (OAT), cryptospermia or non-obstructive azoospermia (NOA). An extremely statistically lower fertilization rate was found in NOA patients. Unexpectedly, no differences were detected in blastocyst formation, euploidy, aneuploidy and mosaicism rates among the four groups. Interestingly, we also found a higher abortion rate comparing NOA to normal semen with an odds ratio of 4.67. In our study no statistically significant differences among the analyzed groups were found, showing little or no effect at all using spermatozoa from different semen sources or quality. This may be linked to the oocyte competence of fixing sperm DNA damage and it could be hypothesized that only sperm with a good rate of DNA integrity are able to fertilize the oocyte, explaining why poor quality semen is reflected in a low fertilization rate without effect on ploidy.

Published
2022

22. Evading the Patronage Trap: Interest Organizations and Policymaking in Mexico

Author

Palmer-Rubin, Brian Dale

Subjects
Political science, Latin American studies, clientelism, development policy, interest representation, Mexico, policymaking
Abstract

This study analyzes the participation of Mexican agricultural and small-business organizations in policymaking. Despite the recent focus in the literature on representation of individual citizens—either through party linkages or participatory institutions—the present focus is on the organizations that exist to represent collective interests of small-scale farmers and small-business owners. I analyze the factors that lead some of these organizations to lend voice to the sectors that they represent in the programmatic policies that shape sectoral competitiveness, others to focus their efforts on extracting distributive benefits from the state, and others to be excluded from policymaking processes entirely. While existing research stresses the effect of poverty on demand for patronage, I identify two factors—membership conditions and electoral competition—that can supersede class pressures, permitting organizations to evade clientelistic linkages with political parties and garner effective policy voice.First, the ability of organizations to independently recruit, retain and mobilize members frees organizations from pressure to enter into dependent linkages with political parties. While such linkages offer particularistic benefits that organization leaders can repurpose as selective benefits to spur member participation, they route organizations into the patronage trap, a self-reproducing cycle in which organizations become specialized for distributive demand making. These linkages convert leaders into electoral brokers and force organizations to forgo protest, lobbying, and other forms of political participation in favor of electoral mobilization, making them ill suited for programmatic demand making. I develop this argument using case studies of economic interest organizations in three Mexican states. Survey analysis of organizations in all Mexican states confirms that independent resource flows and the capacity to generate selective benefits—indicators of member recruitment capacity—are positively associated with organizations’ breadth of mobilization strategies and ability to levy programmatic policy demands.Second, I show that the dynamics of electoral competition help explain the degree to which ruling politicians incorporate organizations into the programmatic and distributive policymaking arenas. In the presence of electoral competition, interest organizations can credibly threaten to support an opposition party if the ruling party fails to respond to their policy demands. Thus, electoral competition has two effects on organizational participation: First, it affords organizations leverage to pressure politicians for access to the exclusive programmatic policy arena, when state actors may otherwise prefer to limit organizational participation to the distributive arena. Second, competition incentivizes ruling politicians to incorporate organizations from their non-core constituencies (such as peasant organizations for a right-wing party or business organizations for a left-wing party) into policymaking. I build this theory through case studies of state governments under the control of three different political parties with different relationships to peasant and small-business organizations. I then test the argument in the distributive realm with an analysis of distribution data for state-level small-business subsidies across all 32 Mexican states, allowing me to exploit subnational variation in ruling parties and electoral competition.

Published
2015

23. Modulating oxidative stress and epigenetic homeostasis in preimplantation IVF embryos

Author

Brian Dale, Kay Elder, Patrice Clement, and Yves Menezo

Subjects
0301 basic medicine, Homocysteine, Reproductive Techniques, Assisted, Fertilization in Vitro, Epigenesis, Genetic, 03 medical and health sciences, chemistry.chemical_compound, Mice, 0302 clinical medicine, Animals, Homeostasis, Epigenetics, chemistry.chemical_classification, 030219 obstetrics & reproductive medicine, Methionine, biology, Cell Biology, Methylation, DNA Methylation, Cystathionine beta synthase, Amino acid, Cell biology, Oxidative Stress, 030104 developmental biology, DNA demethylation, Blastocyst, chemistry, biology.protein, Maternal to zygotic transition, Developmental Biology
Abstract

SummaryAssisted reproductive technology is today considered a safe and reliable medical intervention, with healthy live births a reality for many IVF and ICSI treatment cycles. However, there are increasing numbers of published reports describing epigenetic/imprinting anomalies in children born as a result of these procedures. These anomalies have been attributed to methylation errors in embryo chromatin remodelling during in vitro culture. Here we re-visit three concepts: (1) the so-called ‘in vitro toxicity’ of ‘essential amino acids’ before the maternal to zygotic transition period; (2) the effect of hyperstimulation (controlled ovarian hyperstimulation) on homocysteine in the oocyte environment and the effect on methylation in the absence of essential amino acids; and (3) the fact/postulate that during the early stages of development the embryo undergoes a ‘global’ demethylation. Methylation processes require efficient protection against oxidative stress, which jeopardizes the correct acquisition of methylation marks as well as subsequent methylation maintenance. The universal precursor of methylation [by S-adenosyl methionine (SAM)], methionine, ‘an essential amino acid’, should be present in the culture. Polyamines, regulators of methylation, require SAM and arginine for their syntheses. Cystine, another ‘semi-essential amino acid’, is the precursor of the universal protective antioxidant molecule: glutathione. It protects methylation marks against some undue DNA demethylation processes through ten-eleven translocation (TET), after formation of hydroxymethyl cytosine. Early embryos are unable to convert homocysteine to cysteine as the cystathionine β-synthase pathway is not active. In this way, cysteine is a ‘real essential amino acid’. Most IVF culture medium do not maintain methylation/epigenetic processes, even in mouse assays. Essential amino acids should be present in human IVF medium to maintain adequate epigenetic marking in preimplantation embryos. Furthermore, morphological and morphometric data need to be re-evaluated, taking into account the basic biochemical processes involved in early life.

Published
2021

24. CD36 promotes vasculogenic mimicry in melanoma by mediating adhesion to the extracellular matrix

Author

Brian Dale, Claudine S. Bonder, Lisa M. Ebert, Brenton W Ebert, Michaelia P. Cockshell, Danielle P King, Mark O. DeNichilo, Anthony E. Woods, Carmela Martini, Martini, Carmela, DeNichilo, Mark, King, Danielle P, Cockshell, Michaelia P, Ebert, Brenton, Dale, Brian, Ebert, Lisa M, Woods, Anthony, and Bonder, Claudine S

Subjects
CD36 Antigens, 0301 basic medicine, Cancer Research, integrin, Angiogenesis, Integrin, thrombospondin, Metastasis, 03 medical and health sciences, 0302 clinical medicine, laminin, melanoma, Genetics, medicine, tumor microenvironment, Humans, Vasculogenic mimicry, Melanoma, vasculogenic mimicry, RC254-282, Thrombospondin, Matrigel, Tumor microenvironment, Chemistry, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, Cancer, medicine.disease, Extracellular Matrix, Gene Expression Regulation, Neoplastic, Endothelial stem cell, 030104 developmental biology, Oncology, 030220 oncology & carcinogenesis, Cancer cell, Cancer research, Female, Laminin, CD36, Research Article
Abstract

Background The formation of blood vessels within solid tumors directly contributes to cancer growth and metastasis. Until recently, tumor vasculature was thought to occur exclusively via endothelial cell (EC) lined structures (i.e. angiogenesis), but a second source of tumor vasculature arises from the cancer cells themselves, a process known as vasculogenic mimicry (VM). While it is generally understood that the function of VM vessels is the same as that of EC-lined vessels (i.e. to supply oxygen and nutrients to the proliferating cancer cells), the molecular mechanisms underpinning VM are yet to be fully elucidated. Methods Human VM-competent melanoma cell lines were examined for their VM potential using the in vitro angiogenesis assays (Matrigel), together with inhibition studies using small interfering RNA and blocking monoclonal antibodies. Invasion assays and adhesion assays were used to examine cancer cell function. Results Herein we demonstrate that CD36, a cell surface glycoprotein known to promote angiogenesis by ECs, also supports VM formation by human melanoma cancer cells. In silico analysis of CD36 expression within the melanoma cohort of The Cancer Genome Atlas suggests that melanoma patients with high expression of CD36 have a poorer clinical outcome. Using in vitro ‘angiogenesis’ assays and CD36-knockdown approaches, we reveal that CD36 supports VM formation by human melanoma cells as well as adhesion to, and invasion through, a cancer derived extracellular matrix substrate. Interestingly, thrombospondin-1 (TSP-1), a ligand for CD36 on ECs that inhibits angiogenesis, has no effect on VM formation. Further investigation revealed a role for laminin, but not collagen or fibronectin, as ligands for CD36 expressing melanoma cells. Conclusions Taken together, this study suggests that CD36 is a novel regulator of VM by melanoma cancer cells that is facilitated, at least in part, via integrin-α3 and laminin. Unlike angiogenesis, VM is not perturbed by the presence of TSP-1, thus providing new information on differences between these two processes of tumor vascularization which may be exploited to combat cancer progression.

Published
2021
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25. The negative impact of the environment on methylation/epigenetic marking in gametes and embryos: A plea for action to protect the fertility of future generations

Author

Brian Dale, Yves Menezo, and Kay Elder

Subjects
Male, 0301 basic medicine, Food Safety, media_common.quotation_subject, Embryonic Development, Fertility, Endocrine Disruptors, Biology, Epigenesis, Genetic, Mice, 03 medical and health sciences, 0302 clinical medicine, Genetics, medicine, Animals, Humans, Epigenetics, Epigenesis, media_common, 030219 obstetrics & reproductive medicine, business.industry, Pesticide Residues, Embryo, Cell Biology, DNA Methylation, medicine.disease, Premature ovarian failure, Biotechnology, Oxidative Stress, Germ Cells, 030104 developmental biology, Endocrine disruptor, Infertility, Food processing, Life expectancy, Nanoparticles, Environmental Pollutants, Female, business, Developmental Biology
Abstract

Life expectancy has increased since World War II, and this may be attributed to several aspects of modern lifestyles. However, now we are faced with a downturn, which seems to be the result of environmental issues. This paradigm is paralleled with reduced human fertility, decreased sperm quality, increased premature ovarian failure, and diminished ovarian reserve syndromes. Endocrine disruptor chemicals and other toxic chemicals, herbicides, pesticides, plasticizers, to mention a few, are a rising concern in today's environment. Some of these are commonly used in the domestic setting: cleaning material and cosmetics and they have a known impact on epigenesis and imprinting via perturbation of methylation processes. Pollution from polyaromatic hydrocarbons, particulate matter

Published
2019
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26. DAAM1 and PREP are involved in human spermatogenesis

Author

Loredana Di Matteo, Chiara Fasano, Sergio Minucci, Antonio Agostino Sinisi, Ismene Serino, Brian Dale, Massimo Venditti, Venditti, Massimo, Fasano, Chiara, Minucci, Sergio, Serino, Ismene, Sinisi, Antonio Agostino, Dale, Brian, and DI MATTEO, Loredana

Subjects
Adult, Male, rho GTP-Binding Proteins, Reproductive technology, Mitochondrial Proteins, 03 medical and health sciences, 0302 clinical medicine, Endocrinology, Prolyl endopeptidase, Testis, Genetics, medicine, Humans, Spermatogenesis, Cytoskeleton, Molecular Biology, 030304 developmental biology, 0303 health sciences, DAAM1, 030219 obstetrics & reproductive medicine, Sperm Count, biology, DAAM!, PREP, Fertility, Cytoskeleton, Testis, Spermatozoa, Human, Microfilament Proteins, Serine Endopeptidases, Spermatozoa, Testicular sperm extraction, Cell biology, medicine.anatomical_structure, Reproductive Medicine, Asthenozoospermia, Case-Control Studies, Formins, Sperm Motility, biology.protein, Gamete, Animal Science and Zoology, Developmental Biology, Biotechnology, medicine.drug
Abstract

During differentiation of the male gamete, there is a massive remodelling in the shape and architecture of all the cells in the seminiferous epithelium. The cytoskeleton, as well as many associated proteins, plays a pivotal role in this process. To better characterise the factors involved, we analysed two proteins: the formin, dishevelled-associated activator of morphogenesis 1 (DAAM1), which participates in the regulation of actin polymerisation, and the protease, prolyl endopeptidase (PREP), engaged in microtubule-associated processes. In our previous studies we demonstrated their involvement in cytoskeletal dynamics necessary for correct postnatal development of the rat testis. Here, we used samples of testicular tissue obtained from infertile men by testicular sperm extraction and the spermatozoa of asthenoteratozoospermic patients. By western blot and immunofluorescent analysis, we found that DAAM1 and PREP expression and localisation were impaired in both the testis and spermatozoa, and in particular in the midpiece as well as in the principal and end-pieces of the flagella, as compared with spermatozoa of normospermic men. Our results provide new knowledge of the dynamics of spermatogenesis, raising the possibility of using DAAM1 and PREP as new markers of normal fertility.

Published
2020

27. Platelets disrupt vasculogenic mimicry by cancer cells

Author

Emma J. Thompson, Carmela Martini, Emma C. Josefsson, Stephanie R. Hyslop, Brian Dale, Claudine S. Bonder, Anthony E. Woods, Lisa M. Ebert, Michaelia P. Cockshell, Martini, Carmela, Thompson, Emma J, Hyslop, Stephanie R, Cockshell, Michaelia P, Dale, Brian J, Ebert, Lisa M, Woods, Anthony E, Josefsson, Emma C, and Bonder, Claudine S

Subjects
0301 basic medicine, Blood Platelets, Male, Angiogenesis, lcsh:Medicine, Apoptosis, Breast Neoplasms, Article, Metastasis, Neovascularization, 03 medical and health sciences, Mice, 0302 clinical medicine, Cell Line, Tumor, Neoplasms, medicine, Animals, Platelet, Vasculogenic mimicry, Neoplasm Metastasis, lcsh:Science, Melanoma, Mice, Inbred BALB C, Multidisciplinary, Aspirin, Neovascularization, Pathologic, business.industry, lcsh:R, Cancer, medicine.disease, tumour vasculature, Endothelial stem cell, 030104 developmental biology, Mechanisms of disease, 030220 oncology & carcinogenesis, Cancer cell, platelets, Cancer research, cancer cells, lcsh:Q, Female, medicine.symptom, business, Neoplasm Transplantation, Tumour angiogenesis
Abstract

Tumour vasculature supports the growth and progression of solid cancers with both angiogenesis (endothelial cell proliferation) and vasculogenic mimicry (VM, the formation of vascular structures by cancer cells themselves) predictors of poor patient outcomes. Increased circulating platelet counts also predict poor outcome for cancer patients but the influence of platelets on tumour vasculature is incompletely understood. Herein, we show with in vitro assays that platelets did not influence angiogenesis but did actively inhibit VM formation by cancer cell lines. Both platelet sized beads and the releasates from platelets were partially effective at inhibiting VM formation suggesting that direct contact maximises the effect. Platelets also promoted cancer cell invasion in vitro. B16F10 melanomas in Bcl-xPlt20/Plt20 thrombocytopenic mice showed a higher content of VM than their wildtype counterparts while angiogenesis did not differ. In a xenograft mouse model of breast cancer with low-dose aspirin to inactivate the platelets, the burden of MDA-MB-231-LM2 breast cancer cells was reduced and the gene expression profile of the cancer cells was altered; but no effect on tumour vasculature was observed. Taken together, this study provides new insights into the action of platelets on VM formation and their involvement in cancer progression.

Published
2020

28. In Vitro Reversal of the Anti-Aggregant Effect of Ticagrelor Using Untreated Platelets

Author

Jeffrey S. Ginsberg, Vinai Bhagirath, Tim A. C. de Vries, John W. Eikelboom, Ke Xu, Noel C. Chan, Paul C Kruger, Brian Dale, Jack Hirsh, Kruger, Paul C, Hirsh, Jack, Bhagirath, Vinai C, Xu, Ke, Dale, Brian, de Vries, Tim AC, Ginsberg, Jeffrey S, Eikelboom, John W, and Chan, Noel C

Subjects
Adult, Blood Platelets, Male, Risk, Ticagrelor, Acute coronary syndrome, Platelet Aggregation, aspirin, Hemorrhage, Platelet Transfusion, 030204 cardiovascular system & hematology, ticagrelor, Young Adult, 03 medical and health sciences, 0302 clinical medicine, medicine, Humans, Platelet, 030212 general & internal medicine, Acute Coronary Syndrome, Cells, Cultured, Platelet-Rich Plasma, business.industry, aggregation, Thrombosis, Hematology, medicine.disease, Adenosine, Healthy Volunteers, Adenosine Diphosphate, Platelet transfusion, Apheresis, medicine.anatomical_structure, Anesthesia, platelet transfusion, Female, business, Platelet Aggregation Inhibitors, medicine.drug, Artery
Abstract

Background Ticagrelor is an anti-platelet agent that is indicated for prevention of thrombosis after acute coronary syndrome or intra-coronary artery stent implantation, but it increases the risk of bleeding. Platelet transfusion has the potential to treat or prevent bleeding in patients taking ticagrelor, but the optimal quantity of platelets and timing of administration have not been fully defined. Methods and Results Ten healthy subjects took ticagrelor in combination with acetylsalicylic acid for 5 days, and had blood collected prior to treatment and at 2, 10, 24, 48, 72 and 96 hours after the last doses. The potential of platelet transfusion to prevent or reverse bleeding was evaluated by mixing subject and donor platelet-rich plasma in vitro in nine different proportions, and measuring adenosine diphosphate-mediated aggregation by light transmission aggregometry. Spontaneous offset of the anti-aggregant effect of ticagrelor occurred gradually and was complete at 72 hours after the last dose. The addition of donor platelets enhanced the recovery. The addition of the equivalent of six apheresis platelet units produced a 50% relative reversal at 10 hours, and > 90% reversal at 24 hours. Conclusion Donor platelets enhance reversal of the anti-aggregant effect of ticagrelor in vitro. Donor platelets given in clinically relevant amounts partially reversed ticagrelor at 10 hours after the last dose, and almost fully reversed ticagrelor at 24 hours. The results inform on the potential to reverse ticagrelor in patients who develop bleeding or require emergency surgery.

Published
2018
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29. Metabolic enhancers supporting 1-carbon cycle affect sperm functionality: an in vitro comparative study

Author

Brian Dale, Alessandra Gallo, Maurizio Dattilo, Elisabetta Tosti, Raffaele Boni, Yves Menezo, and Giuseppe Coppola

Subjects
0301 basic medicine, Male, Antioxidant, medicine.medical_treatment, Intracellular pH, lcsh:Medicine, Hypotaurine, medicine.disease_cause, Article, Andrology, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, medicine, Animals, Humans, Urochordata, lcsh:Science, Sperm plasma membrane, chemistry.chemical_classification, Membrane Potential, Mitochondrial, Reactive oxygen species, 030219 obstetrics & reproductive medicine, Multidisciplinary, lcsh:R, Glutathione, Hydrogen-Ion Concentration, Sperm, Spermatozoa, Carbon, Oxidative Stress, 030104 developmental biology, chemistry, Sperm Motility, Cattle, lcsh:Q, Lipid Peroxidation, Reactive Oxygen Species, Oxidative stress
Abstract

The sperm plasma membrane is a sensitive target to oxidative stress. The most representative reactive oxygen species (ROS) scavengers in the genital tract, hypotaurine and glutathione, require, for their synthesis, cysteine whose availability is associated with the 1-carbon cycle (1-CC). Human, bovine and ascidian spermatozoa were incubated with compounds supporting the 1-CC (Vitamin B6, Methylcobalamin, 5 Methyl Tetrahydrofolate, Zinc Bisglycinate and N-acetyl-cysteine) (TRT) and compared to the effects induced solely by N-acetyl-cysteine (NAC). In control groups (CNTRL), spermatozoa were incubated with medium alone. After 90 and 180 minutes of incubation, the mitochondrial membrane potential (ΔΨM) in TRT and NAC was significantly (P 2DCFDA evaluation, ROS production differed between species whereas, at 2-OH Ethidium, it significantly decreased in bovine TRT group. Intracellular pH (pHi) did not significantly vary in relation to treatment. In ascidian spermatozoa, the NAC supplementation decreased external pH, which in turn brought to a pHi lowering. Buffering seawater with NaHCO3 reversed the beneficial effects of N-acetyl-cysteine supplementation. In conclusion, both fully supporting the 1-CC and treatment with N-acetyl-cysteine alone improved kinetics, ΔΨM and ROS production in mammalian sperm demonstrating for the first time the direct in vitro effects of these compounds on sperm functionality.

Published
2018
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31. Time to re-evaluate ART protocols in the light of advances in knowledge about methylation and epigenetics: an opinion paper

Author

Brian Dale, Yves Menezo, and Kay Elder

Subjects
Male, 0301 basic medicine, Pediatric Obesity, Biomedical Research, Reproductive Techniques, Assisted, Autism Spectrum Disorder, Biochemical Process, Reproductive technology, Computational biology, Endocrine Disruptors, Biology, Models, Biological, DNA sequencing, Epigenesis, Genetic, Embryo Culture Techniques, Mice, 03 medical and health sciences, 0302 clinical medicine, Species Specificity, Health Transition, Plasticizers, Pregnancy, Animals, Humans, Epigenetics, Imprinting (psychology), Genetics, 030219 obstetrics & reproductive medicine, Obstetrics and Gynecology, Embryo, General Medicine, Methylation, DNA Methylation, Oxidative Stress, 030104 developmental biology, Reproductive Medicine, embryonic structures, DNA methylation, Ectogenesis, Female
Abstract

DNA methylation is a biochemical process that modifies gene expression without changing the underlying DNA sequence, and this represents the molecular basis for imprinting and epigenetics. Recent reports have revealed alterations in DNA methylation profiles in the placenta of babies born from assisted reproductive technologies (ART). This supports several previous observations that suggested an increase in the prevalence of imprinting diseases following ART treatment, and also fits our observations regarding the metabolism and requirements of early human embryos. Human embryo culture media (HECM) are currently formulated according to requirements based on the mouse embryo model, and in fact need to pass the Mouse Embryo Assay test in order to be accepted by the relevant authorities, despite the fact that physiological (especially the time necessary to reach genomic activation) and biochemical requirements of mouse and human embryos are quite different. This commentary aims to explain some of the discrepancies, and emphasize why human embryo metabolism tells us that the composition of HECM, as well as the role of the MEA as a unique model, should be re-evaluated.

Published
2017
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32. Distribution of uranium and fluoride in some two-phase solvent systems

Author

Waite, Brian Dale Anthony

Subjects
540
Abstract

Studies have been made of the extraction from aqueous solution of nitric and hydrofluoric acids, alone and in the presence of each other and, where relevant of hydrochloric acid, into di-(2-ethyl hexyl)phosphate, tri-n-butyl phosphate and tri-n-octylamine. Also, similar studies have been made of the extraction of uranium in the presence of hydrofluoric and nitric acids into the same acidic, neutral and basic organic solvents. In all cases, the practical work has taken the form of equilibrium experiments made under carefully controlled conditions and analysis of the resulting aqueous and organic phases. The organic solvents have been used either alone or as solutions in various inert diluents such as kerosene, benzene or xylene and the aqueous solutions have covered a very wide range of concentrations. From the results of these experiments, deductions have been made regarding the mechanisms of the extraction processes and the nature of the species taken up into the organic media. Equilibrium constants are given and, where sufficient data is available, stability constants have been calculated. The extraction of the mineral acids into di-(2-ethyl hexyl)phosphate and tributyl phosphate is found to be similar. With dilute aquwous solutions, one mole of acid is taken up per mole of extractant and the acid is probably hydrogen bonded to the phosphoryl oxygen. At higher aqueous concentrations, more acid is extracted and possible explanations of this are offered. With tri-octylamine, the acids are extracted as the amine salts R3NH. NO3 or R3NH. HF2 but again more acid than expected is taken up from concentrated aqueous solutions. Uranium is extracted into tributyl phosphate in the presence of nitric or hydrochloric acids but not at all in the presence of hydrofluoric acid and possible explanations are offered for this. With di-(2-ethyl hexyl)phosphate and tri-n-octylamine uranium is extracted in the presence of all acids and it would appear from the results that this is a simple ion exchange process, UO2 2+ exchanging with H+ in the former case and UO2F3 - exchanging with the anion in the latter case.

Published
1964

34. Combined Raman and polarization sensitive holographic imaging for a multimodal label-free assessment of human sperm function

Author

Annalisa De Angelis, Brian Dale, Loredana Di Matteo, Maria Antonietta Ferrara, Anna Chiara De Luca, Gianfranco Coppola, Giuseppe Coppola, and Laura Siani

Subjects
0301 basic medicine, Male, Acrosome reaction, Holography, lcsh:Medicine, Spectrum Analysis, Raman, Article, 03 medical and health sciences, symbols.namesake, 0302 clinical medicine, Capacitation, Microscopy, Humans, lcsh:Science, Multidisciplinary, Birefringence, Chemistry, urogenital system, Acrosome Reaction, lcsh:R, Holographic imaging, Sperm, Spermatozoa, Healthy Volunteers, Semen Analysis, 030104 developmental biology, Microscopy, Fluorescence, Infertility, Raman spectroscopy, Biophysics, symbols, Birifringence, lcsh:Q, Microscopy, Polarization, Sperm Capacitation, 030217 neurology & neurosurgery, Digital holography, label-free imaging
Abstract

Raman microspectroscopy (RM) and polarization sensitive digital holographic imaging (PSDHI) are valuable analytical tools in biological and medical research, allowing the detection of both biochemical and morphological variations of the sample without labels or long sample preparation. Here, using this multi-modal approach we analyze in vitro human sperm capacitation and the acrosome reaction induced by heparin. The multimodal microscopy provides morphofunctional information that can assess the sperms ability to respond to capacitation stimuli (sperm function). More precisely, the birefringence analysis in sperm cells can be used as an indicator of its structural normality. Indeed, digital holography applied for polarization imaging allows for revelation of the polarization state of the sample, showing a total birefringence of the sperm head in non-reacted spermatozoa, and a birefringence localized in the post-acrosomal region in reacted spermatozoa. Additionally, RM allows the detection and spectroscopic characterization of protein/lipid delocalization in the plasma and acrosomal membranes that can be used as valuable Raman biomarkers of sperm function. Interestingly, these spectral variations can be correlated with different time phases of the cell capacitation response. Although further experimentation is required, the proposed multimodal approach could represent a potential label-free diagnostic tool for use in reproductive medicine and the diagnosis of infertility.

Published
2019
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35. A Requirement for ZAK Kinase Activity in Canonical TGF-β Signaling1

Author

Nyati, Shyam, Chator, Areeb, Schinske, Katerina, Gregg, Brandon S, Ross, Brian Dale, and Rehemtulla, Alnawaz

Subjects
Original article
Abstract

The sterile alpha motif and leucine zipper containing kinase ZAK (AZK, MLT, MLK7), is a MAPK-kinase kinase (MKKK). Like most MAPKKKs which are known to activate the c-Jun. amino-terminal kinase (JNK) pathway, ZAK has been shown to participate in the transduction of Transforming growth factor-β (TGF-β)-mediated non-canonical signaling. A role for ZAK in SMAD-dependent, canonical TGF-β signaling has not been previously appreciated. Using a combination of functional genomics and biochemical techniques, we demonstrate that ZAK regulates canonical TGFβRI/II signaling in lung and breast cancer cell lines and may serve as a key node in the regulation of TGFBR kinase activity. Remarkably, we demonstrate that siRNA mediated depletion of ZAK strongly inhibited TGF-β dependent SMAD2/3 activation and subsequent promoter activation (SMAD binding element driven luciferase expression; SBE4-Luc). A ZAK specific inhibitor (DHP-2), dose-dependently activated the bioluminescent TGFBR-kinase activity reporter (BTR), blocked TGF-β induced SMAD2/3 phosphorylation and SBE4-Luc activation and cancer cell-invasion. In aggregate, these findings identify a novel role for the ZAK kinase in canonical TGF-β signaling and an invasive cancer cell phenotype thus providing a novel target for TGF-β inhibition.

Published
2016

36. Simultaneous Holographic Microscopy and Raman Spectroscopy Monitoring of Human Spermatozoa Photodegradation

Author

Maria Antonietta Ferrara, Giuseppe Coppola, Anna Chiara De Luca, Annalisa De Angelis, and Brian Dale

Subjects
Materials science, macromolecular substances, 02 engineering and technology, law.invention, 03 medical and health sciences, symbols.namesake, 020210 optoelectronics & photonics, 0302 clinical medicine, Optics, law, Microscopy, 0202 electrical engineering, electronic engineering, information engineering, Irradiation, Electrical and Electronic Engineering, Spectroscopy, Photodegradation, 030219 obstetrics & reproductive medicine, urogenital system, business.industry, Digital holography, Laser, Atomic and Molecular Physics, and Optics, spermatozoa analysis, Raman spectroscopy, symbols, Biophysics, business, Raman scattering
Abstract

Coupling digital holography with high-specific Raman spectroscopy is an attractive means of identifying biochemical changes in cells by both physical topography and spectroscopy. We have used this approach to simultaneously study biochemical and morphological characteristics of human sperm cells irradiated with green laser radiation. Severe spermatozoa variations associated with a topological redistribution of the sample and a gradual decrease in the Raman signal intensity were detected in a label-free configuration. Importantly, at laser fluences where no morphological alterations were detected (30 MJ/cm2 ), high specific spectral variations were monitored to evaluate the cell photodegradation.

Published
2016
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39. Quantifying immature platelets as markers of increased platelet production after coronary artery bypass grafting surgery

Author

Richard P. Whitlock, Brian Dale, Jeffrey S. Ginsberg, Chunjian Li, Paul C Kruger, Jack Hirsh, Ke Xu, Noel C. Chan, Mark Crowther, John W. Eikelboom, Vinai Bhagirath, Xu, Ke, Chan, Noel C, Hirsh, Jack, Ginsberg, Jeffrey S, Bhagirath, Vinai, Kruger, Paul, Dale, Brian, Crowther, Mark, Whitlock, Richard P, Li, Chunjian, and Eikelboom, John W

Subjects
Blood Platelets, Male, medicine.medical_specialty, Time Factors, immature platelet fraction, Bypass grafting, platelet turnover, 030204 cardiovascular system & hematology, Immature Platelet, Thrombopoiesis, 03 medical and health sciences, 0302 clinical medicine, Risk Factors, Internal medicine, parasitic diseases, Antithrombotic, medicine, Humans, Platelet, cardiovascular diseases, Postoperative Period, Mean platelet volume, Coronary Artery Bypass, immature platelet count, Aged, Aspirin, mean platelet volume, business.industry, Platelet Count, Hematology, General Medicine, Middle Aged, coronary artery bypass, medicine.anatomical_structure, 030220 oncology & carcinogenesis, Cardiology, Female, business, Mean Platelet Volume, Artery, medicine.drug
Abstract

Objectives: An increased rate of platelet production is a possible cause of reduced antithrombotic response to once-daily aspirin. Markers of immature platelets (IPs),such as immature platelet count (IPC), immature platelet fraction (IPF), and mean platelet volume (MPV) might be useful for identifying patients who have an increase in their rate of platelet production. However, their potential as markers of platelet production has not been rigorously evaluated. We aimed to investigate the utility of the IPC, IPF, and MPV as surrogates for increased platelet production using coronary artery bypass grafting (CABG) as a model of enhanced thrombopoiesis. Methods: Daily changes in platelet count, IPC, IPF, and MPV were followed in 45 patients undergoing CABG. Results: The rise in IP markers preceded that in the platelet count. IPC (16% per day increase from nadir) but not IPF or MPV showed a significant and sustained rise,which paralleled the pattern observed with platelet count (18% per day increase from nadir).Conclusions: Of the 3 markers, IPC was the most promising as surrogates for platelet production. Future studies should evaluate the utility of the IPC to identify patientswith cardiovascular disease with reduced response to aspirin who might benefit fromtwice-dailyaspirin. Refereed/Peer-reviewed

Published
2018

40. Mechanistic Basis for the Differential Effects of Rivaroxaban and Apixaban on Global Tests of Coagulation

Author

Alan R. Stafford, Jeffrey I. Weitz, Paul Y. Kim, Calvin H. Yeh, James C. Fredenburgh, Brian Dale, Jack Hirsh, and Beverly A. Leslie

Subjects
Prothrombin time, lcsh:Diseases of the circulatory (Cardiovascular) system, 0303 health sciences, Rivaroxaban, medicine.diagnostic_test, Chemistry, DOAC, coagulation assays, coagulation inhibitors, Inhibition kinetics, 030204 cardiovascular system & hematology, Pharmacology, Differential effects, 03 medical and health sciences, 0302 clinical medicine, Coagulation, lcsh:RC666-701, inhibition kinetics, medicine, Apixaban, Original Article, 030304 developmental biology, medicine.drug, Partial thromboplastin time
Abstract

Rivaroxaban and apixaban are both small molecules that reversibly inhibit factor Xa. Compared with rivaroxaban, apixaban has minimal effects on the prothrombin time and activated partial thromboplastin time. To investigate this phenomenon, we used a factor Xa-directed substrate in a buffer system. Although rivaroxaban and apixaban inhibited factor Xa with similar Ki values at equilibrium, kinetic measurements revealed that rivaroxaban inhibited factor Xa up to 4-fold faster than apixaban (p

Published
2018

41. Polyspermy

Author

Brian Dale

Subjects
0301 basic medicine, 03 medical and health sciences, 030219 obstetrics & reproductive medicine, 030104 developmental biology, 0302 clinical medicine
Published
2018
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44. Laboratory measurement of the direct oral anticoagulants

Author

Brian Dale, John W. Eikelboom, Noel C. Chan, Dale, Brian J, Chan, Noel C, and Eikelboom, John W

Subjects
anticoagulants, Anticoagulant effect, Pyridines, Pyridones, Administration, Oral, 030204 cardiovascular system & hematology, Pharmacology, drugs, Dabigatran, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Rivaroxaban, Edoxaban, medicine, Coagulation testing, Humans, coagulation, Blood Coagulation, Chromatography, High Pressure Liquid, Blood coagulation test, business.industry, Anticoagulants, Hematology, thrombosis, Thiazoles, chemistry, Direct thrombin inhibitor, laboratory haematology, 030220 oncology & carcinogenesis, Pyrazoles, Apixaban, Blood Coagulation Tests, Drug Monitoring, business, medicine.drug
Abstract

Direct oral anticoagulants (DOACs), including the direct thrombin inhibitor, dabigatran, and the direct factor Xa (FXa) inhibitors, rivaroxaban, apixaban and edoxaban, are approved for thromboembolism prevention and treatment. These drugs do not require routine coagulation monitoring but, in some circumstances, measurement of drug level or anticoagulant effect may be necessary. Although traditional coagulation tests lack analytical sensitivity and specificity, they are widely available and inexpensive, and can provide useful information regarding the residual anticoagulant effect of DOACs. Hemoclot® and ecarin-based assays can be used to quantify dabigatran level and calibrated chromogenic anti-FXa assays are suitable for measuring rivaroxaban, apixaban and edoxaban levels, but these tests are not yet widely available. Refereed/Peer-reviewed

Published
2015
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45. Evaluating coagulation tests in patients with atrial fibrillation using direct oral anticoagulants

Author

Vinai Bhagirath, Brian Dale, Noel C. Chan, John W. Eikelboom, Chan, Noel C, Bhagirath, Vinai, Dale, Brian J, and Eikelboom, John W

Subjects
anticoagulants, medicine.medical_specialty, medicine.drug_class, direct oral anticoagulant, Hemorrhage, Dabigatran, chemistry.chemical_compound, Edoxaban, Atrial Fibrillation, Internal Medicine, Coagulation testing, Humans, Medicine, atrial fibrillation, NOACs, coagulation, Blood Coagulation, Rivaroxaban, business.industry, Anticoagulant, Warfarin, Anticoagulants, Atrial fibrillation, Venous Thromboembolism, General Medicine, medicine.disease, stroke, Surgery, Stroke, monitoring, chemistry, Anesthesia, Apixaban, Cardiology and Cardiovascular Medicine, business, laboratory, medicine.drug
Abstract

Four direct oral anticoagulants (dabigatran, rivaroxaban, apixaban, edoxaban) have been shown to be at least as effective and safe as warfarin for the prevention of stroke in atrial fibrillation and the prevention and treatment of venous thromboembolism. Although they are administered in fixed doses without routine coagulation monitoring, measurement of anticoagulant effect or drug levels may be useful to determine if: anticoagulant effect is present in patients who are bleeding or require an urgent procedure or thrombolysis; levels are within usual on-therapy range in patients with recurrent thromboembolism during treatment; and levels are outside of the usual on-therapy range in patients with overdose or with extreme clinical characteristics. Traditional coagulation assays are widely available but lack sensitivity to detect clinically relevant anticoagulant effects, and lack accuracy in quantitating drug levels. Specific drug assays are less widely available but can accurately measure drug levels and should be preferred. Refereed/Peer-reviewed

Published
2015
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48. Evaluation of Pre-analytical Variables in a Commercial Thrombin Generation Assay

Author

Brian Dale, Susan E. Rodgers, Reanuga D. Gopal, Simon J. McRae, Amanda Wong, Elizabeth M. Duncan, Rodgers, Susan E, Wong, Amanda, Gupal, Reanuga D, Dale, Brian J, Duncan, Elizabeth M, and McRae, Simon J

Subjects
centrifugation, Chromatography, Chemistry, Thrombin, Analytical chemistry, Phospholipid, blood coagulation tests, Centrifugation, corn trypsin inhibitor, Hematology, time factors, Thromboplastin, law.invention, Tissue factor, chemistry.chemical_compound, Membrane, thrombin generation assay, law, Reagent, Humans, Blood Coagulation Tests, Filtration, Blood coagulation test, Platelet-poor plasma
Abstract

Background: There is minimal data on the influence of pre-analytical variables on the use of calibrated automated thrombography (CAT), to measure thrombin generation. Objectives: To evaluate the impact of centrifugation methods, time after collection, and contact activation inhibition on the CAT assay performed using two commercial reagents. Methods and Results: Six different methods of plasma separation were examined. Thrombin generation triggered by a 5 pM tissue factor reagent was not greatly affected by plasma separation method,with similar results obtained with all methods apart from single centrifugation and membrane filtration. Membrane filtration increased APTT and is not recommended. Extended double centrifugation at higher speed was required to minimise the impact of residual phospholipid with 1 pM tissue factor trigger, particularly with inhibition of contact activation. The effect of a delay of up to 24 hours in preparing plasma was assessed. No significant difference in results was observed among samples processed between 0.5 and 6 hours after blood collection into plastic Vacuette® tubes. The presence or absence of corn trypsin inhibitor had a significant impact on all parameterswith 1 pM tissue factor trigger, with minor differences seen on Peak and ttPeak results using 5 pM tissue factor. Conclusions: The impact of pre-analytical variables on thrombin generation results is dependent on the concentration of tissue factor in the trigger reagent used. Results with 1 pM tissue factor are particularly sensitive to centrifugation method and contact activation, and standardisation is required to allow large collaborative studies to be performed. Refereed/Peer-reviewed

Published
2014
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49. DNA Methylation Patterns in the Early Human Embryo and the Epigenetic/Imprinting Problems: A Plea for a More Careful Approach to Human Assisted Reproductive Technology (ART)

Author

Brian Dale, Yves Menezo, and Patrice Clement

Subjects
0301 basic medicine, Zygote, medicine.medical_treatment, Cell Culture Techniques, Fertilization in Vitro, Biology, Bioinformatics, Catalysis, Epigenesis, Genetic, lcsh:Chemistry, Inorganic Chemistry, Genomic Imprinting, 03 medical and health sciences, 0302 clinical medicine, Human fertilization, culture conditions, medicine, Humans, Epigenetics, Physical and Theoretical Chemistry, Imprinting (psychology), lcsh:QH301-705.5, Molecular Biology, Spectroscopy, 030219 obstetrics & reproductive medicine, Assisted reproductive technology, In vitro fertilisation, Organic Chemistry, maternal to zygotic transition, Gene Expression Regulation, Developmental, epigenesis, Embryo, General Medicine, Methylation, DNA Methylation, Embryo, Mammalian, Computer Science Applications, Oxidative Stress, 030104 developmental biology, lcsh:Biology (General), lcsh:QD1-999, IVF, DNA methylation, Commentary, methylation, imprinting
Abstract

An increasing number of publications indicate that babies born after IVF (in vitro fertilization) procedures have higher rates of anomalies related to imprinting/epigenetic changes, which may be attributed to suboptimal culture conditions. Appropriate maintenance of DNA methylation during the first few days of an in vitro culture requires a supply of methyl donors, which are lacking in current in vitro culture systems. The absence of protection against oxidative stress in the culture increases the risks for errors in methylation. A decrease in the methylation processes is sometimes observed immediately post fertilization, due to delays that occur during the maternal–zygotic transition period. Care should be exercised in ART (assisted reproductive technology) procedures in order to avoid the risk of generating errors in methylation during the in vitro culture period immediately post fertilization, which has an impact on imprinting/epigenetics. Formulation of IVF culture media needs to be re-assessed in the perspective of current knowledge regarding embryo physiology.

Published
2019
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50. Investigation of ticks and red blood cell parasites of a population of reintroduced mainland tammar wallabies (Notamacropus eugenii eugenii)

Author

Brian Dale, Sophie Petit, B. Matthews, R. Pradhan, Helen P. Waudby, Andy Sharp, Waudby, HP, Petit, S, Matthews, B, Sharp, A, Pradhan, R, and Dale, B

Subjects
0106 biological sciences, education.field_of_study, Tick-borne disease, biology, Population, Amblyomma, Zoology, Wildlife disease, biology.organism_classification, Notamacropus eugenii, medicine.disease, 010603 evolutionary biology, 01 natural sciences, 010601 ecology, Red blood cell, medicine.anatomical_structure, parasitic diseases, Threatened species, medicine, Animal Science and Zoology, education, Ecology, Evolution, Behavior and Systematics, Marsupial
Abstract

Ticks and blood smears were collected from a reintroduced population of threatened tammar wallabies (Notamacropus eugenii eugenii). Ixodes hirsti was common during autumn/winter, and Amblyomma spp. in spring/summer, reflecting the seasonal density of questing A. triguttatum triguttatum. Red blood cell parasites were not detected in the 90 smears analysed. Refereed/Peer-reviewed

Published
2019
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