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2. Single molecule long-read eccDNA sequencing reveals unambiguous and selective transposon activation in Arabidopsis in response to stress, cellular state, and epigenetic processes

Author

Syed Shan-e-Ali Zaidi, Sara Shakir, Devang Mehta, Vu Nguyen, Ruben Gutzat, and Herve Vanderschuren

Abstract

Extrachromosomal circular DNA (eccDNA) has been described in a number of eukaryotic species, and their presence has been shown to enable gene amplification in phenomena as diverse as cancer and herbicide tolerance. A potential role for eccDNA is to serve as a means for transposon mobilization within the genome. However, most eccDNA studies in plants to date have been based on short-read sequencing data which fails at unambiguously identifying true eccDNA forms of genetic and transposable elements. Here, we report the first atlas of full-length eccDNAs for Arabidopsis using the Cider-Seq pipeline based on long-read sequencing of single molecules. Our dataset was validated by analysing eccDNAs of heat-stressed plants, thereby sequencing full-length eccDNA forms of the well-known heat-responsive ONSEN transposon. Our results show that more evolutionarily recent loci of ONSEN transposon produce greater numbers of eccDNAs upon heat-stress. We identified eccDNAs generated from loci of the transposon superfamily RC/Helitron as the most abundant eccDNAs in Arabidopsis. Profiling of eccDNAs from two cell types displaying altered DNA methylation patterns enabled the identification of new active TE loci such as VANDAL5A, ATCOPIA58 and ATREP19 in the shoot apical meristem, and ATCOPIA53, ENDOVIR1 and TA11 in calli tissues. Unexpectedly analysis of mutants in the DNA methylation pathways revealed that eccDNA formation from several retrotransposon loci is induced in the absence of active DNA demethylase ROS1. Together, our study provides an important resource to investigate the function of eccDNAs and the impact of DNA methylation in their regulation.

Published
2023
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4. Profiling of eccDNAs in Arabidopsis indicates shift in population of TE-derived eccDNAs in response to stress, cellular state,and epigenetic processes

Author

Herve Vanderschuren, Syed Shan-e-Ali Zaidi, Sara Shakir, Devang Mehta, Vu Nguyen, and Ruben Gutzat

Abstract

Evidence for the existence of extrachromosomal circular DNA (eccDNA) was presented decades ago, but only recent technological advancements have allowed a better characterization of eccDNA, including their crucial role in human pathogenesis, which is to increase the copy number and availability of oncogenes. However, the current eccDNA studies are based on short-read sequencing technologies and have limitations in accessing the integrity and abundance of eccDNA populations. Here we provide the eccDNA profiles and the landscape of active transposons in various Arabidopsis tissues, including meristematic cells sorted by fluorescence-activated nuclei, using high-accuracy long-read circular consensus sequencing. Comparative analysis of eccDNA profiles in actively dividing tissues and heat-stressed seedlings was also instrumental to identify known and previously unknown eccDNA-active loci. In-depth analysis of eccDNAs originating from ONSEN loci indicated preferential mobilization from young transposon loci. Our dataset also identified eccDNAs generated from loci of the superfamily RC/Helitrons as the most abundant eccDNAs in Arabidopsis. Profiling of eccDNA populations in selected Arabidopsis mutants of the DNA methylation pathways revealed that eccDNA formation from several retrotransposon loci is induced in the absence of active DNA demethylase ROS1. Together, these eccDNA datasets provide a useful plant genomics resource with the identification of eccDNA-active genomic loci that could help advancing our understanding of eccDNA biogenesis and functions in eukaryotes.

Published
2022
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5. Recommendations for empowering early career researchers to improve research culture and practice

Author

Brianne A. Kent, Constance Holman, Emmanuella Amoako, Alberto Antonietti, James M. Azam, Hanne Ballhausen, Yaw Bediako, Anat M. Belasen, Clarissa F. D. Carneiro, Yen-Chung Chen, Ewoud B. Compeer, Chelsea A. C. Connor, Sophia Crüwell, Humberto Debat, Emma Dorris, Hedyeh Ebrahimi, Jeffrey C. Erlich, Florencia Fernández-Chiappe, Felix Fischer, Małgorzata Anna Gazda, Toivo Glatz, Peter Grabitz, Verena Heise, David G. Kent, Hung Lo, Gary McDowell, Devang Mehta, Wolf-Julian Neumann, Kleber Neves, Mark Patterson, Naomi C. Penfold, Sophie K. Piper, Iratxe Puebla, Peter K. Quashie, Carolina Paz Quezada, Julia L. Riley, Jessica L. Rohmann, Shyam Saladi, Benjamin Schwessinger, Bob Siegerink, Paulina Stehlik, Alexandra Tzilivaki, Kate D. L. Umbers, Aalok Varma, Kaivalya Walavalkar, Charlotte M. de Winde, Cecilia Zaza, Tracey L. Weissgerber, Molecular cell biology and Immunology, AII - Cancer immunology, and CCA - Cancer biology and immunology

Subjects
Research Report, Life Sciences & Biomedicine - Other Topics, Biochemistry & Molecular Biology, Science & Technology, General Immunology and Microbiology, Research, Scientific Reform, General Neuroscience, Política Científica, SCIENCE, Información Científica, Research Personnel, General Biochemistry, Genetics and Molecular Biology, Transferencia de Información, Information Transfer, Research Culture, Investigación, Research Practice, Humans, Power, Psychological, General Agricultural and Biological Sciences, Life Sciences & Biomedicine, Biology, Early Career Researchers, Uncategorized
Abstract

Early career researchers (ECRs) are important stakeholders leading efforts to catalyze systemic change in research culture and practice. Here, we summarize the outputs from a virtual unconventional conference (unconference), which brought together 54 invited experts from 20 countries with extensive experience in ECR initiatives designed to improve the culture and practice of science. Together, we drafted 2 sets of recommendations for (1) ECRs directly involved in initiatives or activities to change research culture and practice; and (2) stakeholders who wish to support ECRs in these efforts. Importantly, these points apply to ECRs working to promote change on a systemic level, not only those improving aspects of their own work. In both sets of recommendations, we underline the importance of incentivizing and providing time and resources for systems-level science improvement activities, including ECRs in organizational decision-making processes, and working to dismantle structural barriers to participation for marginalized groups. We further highlight obstacles that ECRs face when working to promote reform, as well as proposed solutions and examples of current best practices. The abstract and recommendations for stakeholders are available in Dutch, German, Greek (abstract only), Italian, Japanese, Polish, Portuguese, Spanish, and Serbian. Instituto de Patología Vegetal Fil: Kent, Brianne A. Simon Fraser University. Department of Psychology; Canadá Fil: Holman, Constance. Universitätsmedizin Berlin. BIH QUEST Center for Responsible Research. Berlin Institute of Health at Charité; Alemania Fil: Amoako, Emmanuella. Cape Coast Teaching Hospital. Department of Paediatrics and Child Health; Ghana Fil: Amoako, Emmanuella. University of Cape Coast. School of Medicine. Department of Paediatrics and Child Health; Ghana Fil: Antonietti, Alberto. Politecnico di Milano. Department of Electronics, Information and Bioengineering; Italia Fil: Azam, James M. Stellenbosch University. DSI-NRF Center of Excellence in Epidemiological Modelling and Analysis. Department of Mathematics; Sudáfrica Fil: Ballhausen, Hanne. Universitätsmedizin Berlin. BIH QUEST Center for Responsible Research. Berlin Institute of Health at Charité; Alemania Fil: Fil: Ballhausen, Hanne. Universitätsmedizin Berlin. Department of Paediatric Endocrinology and Diabetes, Charité; Alemania Fil: Bediako, Yaw . University of Ghana. West African Centre for Cell Biology of Infectious Pathogens; Ghana Fil: Belasen, Anat M. Cornell University. Society for Conservation Biology. Department of Ecology and Evolutionary Biology; Estados Unidos Fil: Carneiro, Clarissa F. D. Federal University of Rio de Janeiro. Institute of Medical Biochemistry Leopoldo de Meis; Brasil Fil: Chung Chen, Yen. New York University. Department of Biology; Estados Unidos Fil: Debat, Humberto Julio. Instituto Nacional de Tecnología Agropecuaria (INTA). Instituto de Patología Vegetal; Argentina Fil: Debat, Humberto Julio. Consejo Nacional de Investigaciones Científicas y Técnicas. Unidad de Fitopatología y Modelización Agrícola (UFyMA); Argentina Fil: Weissgerber, Tracey L. Universitätsmedizin Berlin. BIH QUEST Center for Responsible Research. Berlin Institute of Health at Charité; Alemania

Published
2022
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6. Closing the protein gap in plant chronobiology

Author

R. Glen Uhrig, Johanna Krahmer, and Devang Mehta

Subjects
Chronobiology Phenomena, Proteomics, biology, Arabidopsis Proteins, Systems biology, fungi, Quantitative proteomics, Circadian clock, Arabidopsis, Cell Biology, Plant Science, Computational biology, biology.organism_classification, Mass Spectrometry, Transcriptome, Gene Expression Regulation, Plant, Circadian Clocks, Proteome, Genetics, Arabidopsis thaliana, DNA microarray, Diel vertical migration
Abstract

Our modern understanding of diel cell regulation in plants stems from foundational work in the late 1990s that analysed the dynamics of selected genes and mutants in Arabidopsis thaliana. The subsequent rise of transcriptomics technologies such as microarrays and RNA sequencing has substantially increased our understanding of anticipatory (circadian) and reactive (light- or dark-triggered) diel events in plants. However, it is also becoming clear that gene expression data fail to capture critical events in diel regulation that can only be explained by studying protein-level dynamics. Over the past decade, mass spectrometry technologies and quantitative proteomic workflows have significantly advanced, finally allowing scientists to characterise diel protein regulation at high throughput. Initial proteomic investigations suggest that the diel transcriptome and proteome generally lack synchrony and that the timing of daily regulatory events in plants is impacted by multiple levels of protein regulation (e.g., post-translational modifications [PTMs] and protein-protein interactions [PPIs]). Here, we highlight and summarise how the use of quantitative proteomics to elucidate diel plant cell regulation has advanced our understanding of these processes. We argue that this new understanding, coupled with the extraordinary developments in mass spectrometry technologies, demands greater focus on protein-level regulation of, and by, the circadian clock. This includes hitherto unexplored diel dynamics of protein turnover, PTMs, protein subcellular localisation and PPIs that can be masked by simple transcript- and protein-level changes. Finally, we propose new directions for how the latest advancements in quantitative proteomics can be utilised to answer outstanding questions in plant chronobiology.

Published
2021
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9. Integrated Systems-Level Proteomics and Metabolomics Reveals the Diel Molecular Landscape of Diverse Kale Cultivars

Author

Sabine Scandola, Devang Mehta, Brigo Castillo, Nicholas Boyce, and R. Glen Uhrig

Abstract

Kale are a group of diverseBrassicaceaespecies that are nutritious leafy greens consumed for their abundance of vitamins and micronutrients. Typified by their curly, serrated and/or wavy leaves, kale varieties have been primarily defined based on their leaf morphology and geographic origin, despite having complex genetic backgrounds. Kale is a very promising crop for vertical farming due to its high nutritional content; however, being a non-model organism, foundational, systems-level analyses of kale are lacking. Previous studies in kale have shown that time-of-day harvesting can affect its nutritional composition. Therefore, to gain a systems-level diel understanding of kale across its wide-ranging and diverse genetic landscape, we selected nine publicly available and commercially grown kale cultivars for growth under near-sunlight LED light conditions ideal for vertical farming. We then analyzed changes in morphology, growth and nutrition using a combination of phenomics, proteomics and metabolomics. As the diel molecular activities of plants drive their daily growth and development, ultimately determining their productivity as a crop, we harvested kale leaf tissue at both end-of-day (ED) and end-of-night (EN) time-points for all molecular analyses. Our results reveal that diel proteome and metabolome signatures divide the selected kale cultivars into two distinct groups, defined by their amino acid and sugar content, along with significant proteome differences involving carbon and nitrogen metabolism, mRNA splicing, protein translation and light harvesting. Together, our multi-cultivar, multi-omic analysis provides robust quantitative insights into the molecular underpinnings of the diel growth and development landscape of kale, significantly advancing our fundamental understanding of this nutritious leafy green super-food for next-generation horticulture / vertical farming applications.

Published
2022
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10. Twelve Principles Trainees, PIs, Departments, and Faculties Can Use to Reduce Bias and Discrimination in STEM

Author

Alexandra N. Davis, Devang Mehta, and Lisa M. Willis

Subjects
General Chemical Engineering, media_common.quotation_subject, Chemistry, Multidisciplinary, Immigration, DIVERSITY, Face (sociological concept), 010402 general chemistry, 01 natural sciences, Indigenous, Representation (politics), STEREOTYPES, Set (psychology), QD1-999, media_common, Science & Technology, 010405 organic chemistry, ME, Lived experience, SUCCESS, General Chemistry, Unconscious bias, PERFORMANCE, 0104 chemical sciences, Chemistry, Physical Sciences, GENDER, Psychology, Social psychology, Research Article
Abstract

There is an overwhelming amount of evidence demonstrating that people from marginalized groups, including women, racialized and Indigenous peoples, people with disabilities, immigrants, and LGBTQ+ individuals, continue to face substantial discrimination in STEM, manifested as both overt bias and unconscious bias. These biases result in discrimination against individuals in marginalized groups, and independent biases collectively contribute to a culture that systematically discriminates against people from marginalized groups. Representation from marginalized groups in postsecondary degrees in natural science and engineering has not substantially improved in over a decade. A set of 10 concrete principles are presented that trainees, principle investigators, departments, and faculties can use to enhance the participation and lived experiences of people in marginalized groups in STEM., Steps to reduce bias toward and promote retention of marginalized peoples need to be active and purposeful in order to increase diversity at all stages in STEM fields.

Published
2020

11. Full-length sequencing of circular DNA viruses and extrachromosomal circular DNA using CIDER-Seq

Author

Syed Shan-e-Ali Zaidi, Luc Cornet, Hervé Vanderschuren, Devang Mehta, and Matthias Hirsch-Hoffmann

Subjects
Biochemistry & Molecular Biology, Sequence analysis, DNA repair, DIVERSITY, Sequence assembly, Computational biology, Biology, Extrachromosomal circular DNA, Genome, Biochemical Research Methods, General Biochemistry, Genetics and Molecular Biology, law.invention, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Plasmid, law, ECCDNA, Polymerase chain reaction, 030304 developmental biology, 0303 health sciences, Science & Technology, CD-HIT, chemistry, Life Sciences & Biomedicine, 030217 neurology & neurosurgery, DNA
Abstract

Circular DNA is ubiquitous in nature in the form of plasmids, circular DNA viruses, and extrachromosomal circular DNA (eccDNA) in eukaryotes. Sequencing of such molecules is essential to profiling virus distributions, discovering new viruses and understanding the roles of eccDNAs in eukaryotic cells. Circular DNA enrichment sequencing (CIDER-Seq) is a technique to enrich and accurately sequence circular DNA without the need for polymerase chain reaction amplification, cloning, and computational sequence assembly. The approach is based on randomly primed circular DNA amplification, which is followed by several enzymatic DNA repair steps and then by long-read sequencing. CIDER-Seq includes a custom data analysis package (CIDER-Seq Data Analysis Software 2) that implements the DeConcat algorithm to deconcatenate the long sequencing products of random circular DNA amplification into the intact sequences of the input circular DNA. The CIDER-Seq data analysis package can generate full-length annotated virus genomes, as well as circular DNA sequences of novel viruses. Applications of CIDER-Seq also include profiling of eccDNA molecules such as transposable elements (TEs) from biological samples. The method takes ~2 weeks to complete, depending on the computational resources available. Owing to the present constraints of long-read single-molecule sequencing, the accuracy of circular virus and eccDNA sequences generated by the CIDER-Seq method scales with sequence length, and the greatest accuracy is obtained for molecules

Published
2020
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12. A Proteome-Level Investigation Into Plasmodiophora brassicae Resistance in Brassica napus Canola

Author

Dinesh Adhikary, Devang Mehta, R. Glen Uhrig, Habibur Rahman, and Nat N. V. Kav

Subjects
Science & Technology, plant-pathogen interaction, DEFENSE, Plant Sciences, Brassica napus, clubroot, LIGNIN CONTENT, CABBAGE, calcium binding, CLUBROOT RESISTANCE, PLANT DEHYDRINS, Plant Science, RAPA, proteomics, INFECTION, ARABIDOPSIS-THALIANA, PATHOGEN, Life Sciences & Biomedicine, GENE-EXPRESSION
Abstract

Clubroot of Brassicaceae, an economically important soil borne disease, is caused by Plasmodiophora brassicae Woronin, an obligate, biotrophic protist. This disease poses a serious threat to canola and related crops in Canada and around the globe causing significant losses. The pathogen is continuously evolving and new pathotypes are emerging, which necessitates the development of novel resistant canola cultivars to manage the disease. Proteins play a crucial role in many biological functions and the identification of differentially abundant proteins (DAP) using proteomics is a suitable approach to understand plant–pathogen interactions to assist in the development of gene specific markers for developing clubroot resistant (CR) cultivars. In this study, P. brassicae pathotype 3 (P3H) was used to challenge CR and clubroot susceptible (CS) canola lines. Root samples were collected at three distinct stages of pathogenesis, 7−, 14−, and 21-days post inoculation (DPI), protein samples were isolated, digested with trypsin and subjected to liquid chromatography with tandem mass spectrometry (LC-MS/MS) analysis. A total of 937 proteins demonstrated a significant (q-value < 0.05) change in abundance in at least in one of the time points when compared between control and inoculated CR-parent, CR-progeny, CS-parent, CS-progeny and 784 proteins were significantly (q < 0.05) changed in abundance in at least in one of the time points when compared between the inoculated- CR and CS root proteomes of parent and progeny across the three time points tested. Functional annotation of differentially abundant proteins (DAPs) revealed several proteins related to calcium dependent signaling pathways. In addition, proteins related to reactive oxygen species (ROS) biochemistry, dehydrins, lignin, thaumatin, and phytohormones were identified. Among the DAPs, 73 putative proteins orthologous to CR proteins and quantitative trait loci (QTL) associated with eight CR loci in different chromosomes including chromosomes A3 and A8 were identified. Proteins including BnaA02T0335400WE, BnaA03T0374600WE, BnaA03T0262200WE, and BnaA03T0464700WE are orthologous to identified CR loci with possible roles in mediating clubroot responses. In conclusion, these results have contributed to an improved understanding of the mechanisms involved in mediating response to P. brassicae in canola at the protein level.

Published
2022
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16. Author response: Vision, challenges and opportunities for a Plant Cell Atlas

Author

Luis C. Romero, Ai My Luong, Jenny C Mortimer, Nicolas L. Taylor, Sergio Alan Cervantes-Pérez, David W. Ehrhardt, Yana Kazachkova, Adrien Burlaocot, Rajiv K. Tripathi, Alfredo Cruz-Ramírez, Nicholas J. Provart, Uwe John, Shou-Ling Xu, Renate A Weizbauer, Mathew G. Lewsey, José M. Palma, R. Glen Uhrig, Asela J. Wijeratne, Maria J. Harrison, William P Dwyer, Alexander T. Borowsky, Yuling Jiao, Kaushal Kumar Bhati, Edoardo Bertolini, Anna Stepanova, Francisco J. Corpas, Fabio Zanini, Pubudu P. Handakumbura, Dominique C. Bergmann, Devang Mehta, Saroj K Sah, Naomi Nakayama, Claire D McWhite, Jahed Ahmed, Dhruv Lavania, Gazala Ameen, Mather A Khan, Marc Libault, Gergo Palfalvi, Seung Y. Rhee, Laura E. Bartley, Vaishali Arora, Cesar L. Cuevas-Velazquez, Josh T. Cuperus, Benjamin Buer, Amir H. Ahkami, Lachezar A. Nikolov, Selena L Rice, Feng Zhao, Ronelle Roth, Ajay Kumar, Atique ur Rehman, Andrew Farmer, Maida Romera-Branchat, Zhi-Yong Wang, Tuan M Tran, Lydia-Marie Joubert, Le Liu, Julia Bailey-Serres, Fabio Gomez-Cano, Ramin Yadegari, Sanjay Joshi, James Whelan, Batthula Vijaya Lakshmi Vadde, Rachel Shahan, Houlin Yu, Bao-Hua Song, Andrey V Malkovskiy, Arun Kumar, Aaron J. Ogden, Javier Brumos, Xiaohong Zhuang, Oluwafemi Alaba, Harmanpreet Kaur, Tatsuya Nobori, Marisa S. Otegui, Peter H Denolf, Miguel Miñambres Martín, Sakil Mahmud, Tingting Xiang, Lisa I David, Justin W. Walley, Purva Karia, Maite Saura-Sanchez, Pankaj Kumar, Jamie Waese, Ansul Lokdarshi, Suryatapa Ghosh Jha, Sagar Kumar, Matthew M. S. Evans, Hai Ying Yuan, Rajveer Singh, Puneet Paul, Carly A Martin, Robert E. Jinkerson, Dianyi Liu, Rajdeep S. Khangura, Dae Kwan Ko, Tedrick Thomas Salim Lew, Jennifer A N Brophy, Ari Pekka Mähönen, Marija Vidović, Mark-Christoph Ott, Alok Arun, Pinky Agarwal, Pradeep Kumar, Alexandre P. Marand, R. Clay Wright, Moises Exposito-Alonso, Rosangela Sozzani, Tamas Varga, Luigi Di Costanzo, Shyam Solanki, Sixue Chen, Chien-Yuan Lin, Iain C. Macaulay, Tie Liu, Elsa H Quezada-Rodríguez, Trevor M. Nolan, Peter Denolf, Stefania Giacomello, Elizabeth S. Haswell, Nancy George, Noel Blanco-Touriñán, Bruno Contreras-Moreira, Benjamin J. Cole, Abhishek Joshi, Steven P. Briggs, Toshihiro Obata, Kerstin Kaufmann, Kenneth D. Birnbaum, Klaas J. van Wijk, Noah Fahlgren, Kamal Kumar Malukani, Ramesh Katam, Pingtao Ding, Mario A. Arteaga-Vazquez, Marcela K. Tello-Ruiz, Shao-shan Carol Huang, Sunil Kumar Kenchanmane Raju, Venura Herath, George W. Bassel, Christopher R. Anderton, Stefan de Folter, Gary Stacey, and Jie Zhu

Subjects
Engineering, Atlas (topology), business.industry, business, Data science
Published
2021
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17. Empowering Early Career Researchers to Improve Science

Author

Brianne A Kent, Constance Holman, Emmanuella Amoako, Alberto Antonietti, JAMES MBA Azam, Hanne Ballhausen, Yaw Bediako, Anat Belasen, Clarissa França Dias Carneiro, Yen-Chung Chen, Ewoud Compeer, Chelsea Connor, Sophia Crüwell, Humberto Debat, Emma Dorris, Hedyeh Ebrahimi, Jeffrey C Erlich, Florencia Fernández Chiappe, Felix Fischer, Małgorzata Anna Gazda, Toivo Glatz, Peter Grabitz, Verena Heise, David Kent, Hung Lo, Gary Mcdowell, Devang Mehta, Wolf-Julian Neumann, Kleber Neves, Mark Patterson, Naomi Penfold, Sophie K. Piper, Iratxe Puebla, Peter Quashie, Carolina Paz Quezada, Julia Lindsay Riley, Jessica L. Rohmann, Shyam Saladi, Benjamin Schwessinger, Bob Siegerink, Paulina Stehlik, Alexandra Tzilivaki, Kate Umbers, Aalok Varma, Kaivalya Walavalkar, Charlotte M de Winde, Cecilia Zaza, and Tracey Lynn Weissgerber

Abstract

Early career researchers (ECRs) are important stakeholders leading efforts to catalyze systemic change in the conduct and communication of science. Here, we summarize the outputs from a virtual unconventional conference (unconference), which brought together 54 invited experts from 20 countries with extensive experience in ECR initiatives designed to improve science. The event was focused on why ECRs are needed to improve science and the obstacles they face when trying to promote reform. Our discussions also highlighted the additional obstacles that ECRs in countries with limited research funding experience when working to improve the scientific system. We provide the lessons learned from successful ECR-led or ECR-focused initiatives and outline actions that individuals and organizations can take to further support ECRs who are working to improve research culture and practice.

Published
2021
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18. DomainViz: intuitive visualization of consensus domain distributions across groups of proteins

Author

Cameron Ridderikhoff, R. Glen Uhrig, Devang Mehta, and Pascal Schläpfer

Subjects
0106 biological sciences, Biochemistry & Molecular Biology, Protein family, Frequency of occurrence, AcademicSubjects/SCI00010, media_common.quotation_subject, Protein domain, Computational biology, PROSITE, Biology, 01 natural sciences, Domain (software engineering), 03 medical and health sciences, Protein Domains, Sequence Analysis, Protein, Genetics, Amino Acid Sequence, Function (engineering), Databases, Protein, Conserved Sequence, 030304 developmental biology, media_common, 0303 health sciences, Science & Technology, EVOLUTION, Visualization, Web Server Issue, Identification (biology), Life Sciences & Biomedicine, Software, 010606 plant biology & botany
Abstract

The prediction of functional domains is typically among the first steps towards understanding the function of new proteins and protein families. There are numerous databases of annotated protein domains that permit researchers to identify domains on individual proteins of interest. However, it is necessary to perform high-throughput domain searches to gain evolutionary insight into the functions of proteins and protein families. Unfortunately, at present, it is difficult to search for, and visualize domain conservation across multiple proteins and/or multiple groups of proteins in an intuitive manner. Here we present DomainViz, a new web-server that streamlines the identification and visualization of domains across multiple protein sequences. Currently, DomainViz uses the well-established PFAM and Prosite databases for domain searching and assembles intuitive, publication-ready ‘monument valley’ plots (mv-plots) that display the extent of domain conservation along two dimensions: positionality and frequency of occurrence in the input protein sequences. In addition, DomainViz produces a conventional domain-ordering figure. DomainViz can be used to explore the conservation of domains within a single protein family, across multiple families, and across families from different species to support studies into protein function and evolution. The web-server is publicly available at: https://uhrigprotools.biology.ualberta.ca/domainviz., Nucleic Acids Research, 49 (1), ISSN:1362-4962, ISSN:0301-5610

Published
2021

20. Vision, challenges and opportunities for a Plant Cell Atlas

Author

George W. Bassel, Claire D McWhite, Dhruv Lavania, Gazala Ameen, Christopher R. Anderton, Rajiv K. Tripathi, Maria J. Harrison, Josh T. Cuperus, Amir H. Ahkami, William P Dwyer, Bao-Hua Song, Fabio Zanini, Miguel Miñambres Martín, Atique ur Rehman, Cesar L. Cuevas-Velazquez, Ari Pekka Mähönen, Tamas Varga, Gergo Palfalvi, Andrew Farmer, Matthew M. S. Evans, Vaishali Arora, Uwe John, Mathew G. Lewsey, Dominique C. Bergmann, Selena L Rice, Mario A. Arteaga-Vazquez, Dae Kwan Ko, Tedrick Thomas Salim Lew, Jennifer A N Brophy, Jenny C Mortimer, Marc Libault, Bruno Contreras-Moreira, Benjamin J. Cole, Naomi Nakayama, Marcela K. Tello-Ruiz, Ronelle Roth, Laura E. Bartley, Tingting Xiang, Benjamin Buer, Shyam Solanki, Nicolas L. Taylor, Feng Zhao, Shao-shan Carol Huang, Alok Arun, Pinky Agarwal, Marisa S. Otegui, Arun Kumar, Marija Vidović, Pankaj Kumar, Aaron J. Ogden, Sagar Kumar, Puneet Paul, Sergio Alan Cervantes-Pérez, Purva Karia, Stefan de Folter, Kerstin Kaufmann, Gary Stacey, Le Liu, Robert E. Jinkerson, Javier Brumos, Harmanpreet Kaur, Tatsuya Nobori, David W. Ehrhardt, Francisco J. Corpas, Steven P. Briggs, James Whelan, Batthula Vijaya Lakshmi Vadde, Peter H Denolf, Tie Liu, Kamal Kumar Malukani, Elsa H Quezada-Rodríguez, Jahed Ahmed, Hai Ying Yuan, Rajveer Singh, Trevor M. Nolan, Ramesh Katam, Mather A Khan, Jamie Waese, Toshihiro Obata, Ramin Yadegari, Lachezar A. Nikolov, Seung Y. Rhee, Luis C. Romero, Ajay Kumar, Kenneth D. Birnbaum, Nicholas J. Provart, Tuan M Tran, Sakil Mahmud, Maida Romera-Branchat, Pradeep Kumar, Saroj K Sah, Ai My Luong, Alexandre P. Marand, R. Clay Wright, Yana Kazachkova, Moises Exposito-Alonso, Klaas J. van Wijk, Noah Fahlgren, Peter Denolf, Fabio Gomez-Cano, Houlin Yu, Luigi Di Costanzo, Adrien Burlaocot, Alfredo Cruz-Ramírez, Pingtao Ding, Dianyi Liu, Renate A Weizbauer, Suryatapa Ghosh Jha, Jie Zhu, Pubudu P. Handakumbura, Kaushal Kumar Bhati, Edoardo Bertolini, Anna Stepanova, Rachel Shahan, Lisa I David, Justin W. Walley, Lydia-Marie Joubert, Nancy George, Sanjay Joshi, José M. Palma, Rosangela Sozzani, Mark-Christoph Ott, Sixue Chen, Ansul Lokdarshi, Sunil Kumar Kenchanmane Raju, Chien-Yuan Lin, Iain C. Macaulay, Venura Herath, Noel Blanco-Touriñán, Rajdeep S. Khangura, Zhi-Yong Wang, Alexander T. Borowsky, Julia Bailey-Serres, Andrey V Malkovskiy, Xiaohong Zhuang, Oluwafemi Alaba, Yuling Jiao, Abhishek Joshi, Devang Mehta, Maite Saura-Sanchez, Carly A Martin, Stefania Giacomello, Elizabeth S. Haswell, Shou-Ling Xu, R. Glen Uhrig, Asela J. Wijeratne, National Science Foundation (US), Jha, S. G., Borowsky, A. T., Cole, B. J., Fahlgren, N., Farmer, A., Huang, S. C., Karia, P., Libault, M., Provart, N. J., Rice, S. L., Saura-Sanchez, M., Agarwal, P., Ahkami, A. H., Anderton, C. R., Briggs, S. P., Brophy, J. A., Denolf, P., Di Costanzo, L., Exposito-Alonso, M., Giacomello, S., Gomez-Cano, F., Kaufmann, K., Ko, D. K., Kumar, S., Malkovskiy, A. V., Nakayama, N., Obata, T., Otegui, M. S., Palfalvi, G., Quezada-Rodriguez, E. H., Singh, R., Uhrig, R. G., Waese, J., VAN WIJK, K., Wright, R. C., Ehrhardt, D. W., Birnbaum, K. D., Rhee, S. Y., Helsinki Institute of Life Science HiLIFE, and Institute of Biotechnology

Subjects
Life Sciences & Biomedicine - Other Topics, 0106 biological sciences, Engineering, chlamydomonas reinhardtii, Chloroplasts, Plant Cell Atla, 0601 Biochemistry and Cell Biology, maize, 01 natural sciences, Zea may, Plant science, Molecular level, cell biology, Plant Cell Atlas Consortium, Image Processing, Computer-Assisted, Biology (General), single-cell omic, 2. Zero hunger, 0303 health sciences, Atlas (topology), General Neuroscience, Agriculture, General Medicine, Plants, ARABIDOPSIS, C-4 PHOTOSYNTHESIS, Plant Cell Atlas, single-cell omics, Plant development, VOCABULARY, SYSTEMS BIOLOGY, Medicine, location-to-function, Life Sciences & Biomedicine, 4D imaging, QH301-705.5, DATABASE, Science, Plant Development, Translational research, Cellular level, Environmental stewardship, Zea mays, Chloroplast, General Biochemistry, Genetics and Molecular Biology, MECHANISMS, 03 medical and health sciences, Component (UML), Plant Cells, Biology, 030304 developmental biology, General Immunology and Microbiology, business.industry, Feature Article, Computational Biology, Plant, 15. Life on land, 11831 Plant biology, GENE, Data science, science forum, translational research, 13. Climate action, A. thaliana, PLASTIDS, Biochemistry and Cell Biology, business, GENERATION, 010606 plant biology & botany
Abstract

With growing populations and pressing environmental problems, future economies will be increasingly plant-based. Now is the time to reimagine plant science as a critical component of fundamental science, agriculture, environmental stewardship, energy, technology and healthcare. This effort requires a conceptual and technological framework to identify and map all cell types, and to comprehensively annotate the localization and organization of molecules at cellular and tissue levels. This framework, called the Plant Cell Atlas (PCA), will be critical for understanding and engineering plant development, physiology and environmental responses. A workshop was convened to discuss the purpose and utility of such an initiative, resulting in a roadmap that acknowledges the current knowledge gaps and technical challenges, and underscores how the PCA initiative can help to overcome them., National Science Foundation 1916797 David W Ehrhardt, Kenneth D Birnbaum, Seung Yon Rhee; National Science Foundation 2052590 Seung Yon Rhee

Published
2021

22. Quantitative proteome and PTMome analysis ofArabidopsis thalianaroot responses to persistent osmotic and salinity stress

Author

Devang Mehta, Maria Camila Rodriguez, Maryalle Tan, and RG Uhrig

Subjects
2. Zero hunger, 0106 biological sciences, 0303 health sciences, Abiotic stress, 15. Life on land, Biology, biology.organism_classification, 01 natural sciences, Cell biology, Transcriptome, 03 medical and health sciences, 13. Climate action, Acetylation, Proteome, medicine, Phosphorylation, Arabidopsis thaliana, Protein phosphorylation, sense organs, Mannitol, 030304 developmental biology, 010606 plant biology & botany, medicine.drug
Abstract

Abiotic stresses such as drought result in large annual economic losses around the world. As sessile organisms, plants cannot escape the environmental stresses they encounter, but instead must adapt to survive. Studies investigating plant responses to osmotic and/or salt stress have largely focused on short-term systemic responses, leaving our understanding of intermediate to longer-term adaptation (24 h - days) lacking. In addition to protein abundance and phosphorylation changes, evidence suggests reversible lysine acetylation may also be important for abiotic stress responses. Therefore, to characterize the protein-level effects of osmotic and salt stress, we undertook a label-free proteomic analysis ofArabidopsis thalianaroots exposed to 300 mM Mannitol and 150 mM NaCl for 24 h. We assessed protein phosphorylation, lysine acetylation and changes in protein abundance, detecting significant changes in 245, 35 and 107 total proteins, respectively. Comparison with available transcriptome data indicates that transcriptome- and proteome-level changes occur in parallel, while PTMs do not. Further, we find significant changes in PTMs and protein abundance involve different proteins from the same networks, indicating a multifaceted regulatory approach to prolonged osmotic and salt stress. In particular, we find extensive protein-level changes involving sulphur metabolism under both osmotic and salt conditions as well as changes in protein kinases and transcription factors that may represent new targets for drought stress signaling. Collectively, we find that protein-level changes continue to occur in plant roots 24 h from the onset of osmotic and salt stress and that these changes differ across multiple proteome levels.

Published
2020
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23. Quantitative Proteome and PTMome Analysis of Arabidopsis thaliana Root Responses to Persistent Osmotic and Salinity Stress

Author

Maryalle Tan, Maria Camila Rodriguez, Devang Mehta, and RG Uhrig

Subjects
0106 biological sciences, 0301 basic medicine, Proteomics, Physiology, Arabidopsis, Plant Science, Biology, 01 natural sciences, Plant Roots, Salt Stress, Transcriptome, 03 medical and health sciences, Gene Expression Regulation, Plant, Osmotic Pressure, Arabidopsis thaliana, Protein phosphorylation, Phosphorylation, Transcription factor, 2. Zero hunger, Abiotic component, Abiotic stress, Arabidopsis Proteins, Lysine, Acetylation, Cell Biology, General Medicine, 15. Life on land, biology.organism_classification, Cell biology, 030104 developmental biology, 13. Climate action, Proteome, sense organs, Protein Processing, Post-Translational, 010606 plant biology & botany
Abstract

Abiotic stresses such as drought result in large annual economic losses around the world. As sessile organisms, plants cannot escape the environmental stresses they encounter but instead must adapt to survive. Studies investigating plant responses to osmotic and/or salt stress have largely focused on short-term systemic responses, leaving our understanding of intermediate to longer-term adaptation (24 h to d) lacking. In addition to protein abundance and phosphorylation changes, evidence suggests reversible lysine acetylation may also be important for abiotic stress responses. Therefore, to characterize the protein-level effects of osmotic and salt stress, we undertook a label-free proteomic analysis of Arabidopsis thaliana roots exposed to 300 mM mannitol and 150 mM NaCl for 24 h. We assessed protein phosphorylation, lysine acetylation and changes in protein abundance, detecting significant changes in 245, 35 and 107 total proteins, respectively. Comparison with available transcriptome data indicates that transcriptome- and proteome-level changes occur in parallel, while post-translational modifications (PTMs) do not. Further, we find significant changes in PTMs, and protein abundance involve different proteins from the same networks, indicating a multifaceted regulatory approach to prolonged osmotic and salt stress. In particular, we find extensive protein-level changes involving sulfur metabolism under both osmotic and salt conditions as well as changes in protein kinases and transcription factors that may represent new targets for drought stress signaling. Collectively, we find that protein-level changes continue to occur in plant roots 24 h from the onset of osmotic and salt stress and that these changes differ across multiple proteome levels.

Published
2020

24. Library-free BoxCarDIA solves the missing value problem in label-free quantitative proteomics

Author

Sabine Scandola, R. Glen Uhrig, and Devang Mehta

Subjects
Workflow, Computer science, Proteome, Quantitative proteomics, Imputation (statistics), Replicate, Instrumentation (computer programming), Computational biology, Proteomics, Interactome
Abstract

The last decade has seen significant advances in the application of quantitative mass spectrometry-based proteomics technologies to tackle important questions in plant biology. The current standard for quantitative proteomics in plants is the use of data-dependent acquisition (DDA) analysis with or without the use of chemical labels. However, the DDA approach preferentially measures higher abundant proteins, and often requires data imputation due to quantification inconsistency between samples. In this study we systematically benchmarked a recently developed library-free data-independent acquisition (directDIA) method against a state-of-the-art DDA label-free quantitative proteomics workflow for plants. We next developed a novel acquisition approach combining MS1-level BoxCar acquisition with MS2-level directDIA analysis that we call BoxCarDIA. DirectDIA achieves a 33% increase in protein quantification over traditional DDA, and BoxCarDIA a further 8%, without any changes in instrumentation, offline fractionation, or increases in mass-spectrometer acquisition time. BoxCarDIA, especially, offers wholly reproducible quantification of proteins between replicate injections, thereby addressing the long-standing missing-value problem in label-free quantitative proteomics. Further, we find that the gains in dynamic range sampling by directDIA and BoxCarDIA translate to deeper quantification of key, low abundant, functional protein classes (e.g., protein kinases and transcription factors) that are underrepresented in data acquired using DDA. We applied these methods to perform a quantitative proteomic comparison of dark and light grown Arabidopsis cell cultures, providing a critical resource for future plant interactome studies. Our results establish BoxCarDIA as the new method of choice in quantitative proteomics using Orbitrap-type mass-spectrometers, particularly for proteomes with large dynamic range such as that of plants.

Published
2020
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25. Ways to increase equity, diversity and inclusion

Author

Vinodh Ilangovan, Charlotte M. de Winde, Julia L. Riley, Carolina P. Quezada, Devang Mehta, Yaw Bediako, Andy Tay, Tracey L. Weissgerber, Hedyeh Ebrahimi, Florencia Fernandez-Chiappe, and Shyam M Saladi

Subjects
Life Sciences & Biomedicine - Other Topics, Gender Equity, 2019-20 coronavirus outbreak, diversity and inclusion, Coronavirus disease 2019 (COVID-19), QH301-705.5, Science, media_common.quotation_subject, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Social Inclusion, Racism, General Biochemistry, Genetics and Molecular Biology, purl.org/becyt/ford/1 [https], Research Communication, equity, Political science, Biology (General), purl.org/becyt/ford/1.6 [https], Biology, media_common, Publishing, early-career researchers, Science & Technology, Equity (economics), General Immunology and Microbiology, business.industry, General Neuroscience, Cultural Diversity, General Medicine, scientific publishing, Public relations, Research Personnel, peer-review, Editorial, Medicine, Scientific publishing, business, Life Sciences & Biomedicine
Abstract

The eLife Early-Career Advisory Group (ECAG), an international group of early-career researchers committed to improving research culture, calls for radical changes at eLife and other journals to address racism in the scientific community and to make science more diverse and inclusive. Fil: Mehta, Devang. University of Alberta; Canadá Fil: Bediako, Yaw. University Of Ghana; Ghana Fil: De Winde, Charlotte M.. Colegio Universitario de Londres; Reino Unido Fil: Ebrahimi, Hedyeh. No especifíca; Fil: Fernández, Florencia. Consejo Nacional de Investigaciones Científicas y Técnicas. Oficina de Coordinación Administrativa Parque Centenario. Instituto de Investigación en Biomedicina de Buenos Aires - Instituto Partner de la Sociedad Max Planck; Argentina Fil: Ilangovan, Vinodh. University Aarhus; Dinamarca Fil: Paz Quezada, Carolina. Universidad Bernardo O'higgins; Chile Fil: Riley, Julia L.. Dalhousie University Halifax; Canadá Fil: Saladi, Shyam M.. California Institute of Technology; Estados Unidos Fil: Tay, Andy. No especifíca; Fil: Weissgerber, Tracey. No especifíca

Published
2020

26. Phosphate and phosphite have a differential impact on the proteome and phosphoproteome of Arabidopsis suspension cell cultures

Author

Devang Mehta, Maryalle Tan, Pascal Schläpfer, R. Glen Uhrig, William C. Plaxton, Mina Ghahremani, and María Pérez-Fernández

Subjects
0106 biological sciences, 0301 basic medicine, Proteomics, Phosphites, Proteome, Cell Respiration, Arabidopsis, chemistry.chemical_element, Plant Science, 01 natural sciences, Phosphates, 03 medical and health sciences, chemistry.chemical_compound, Genetics, Arabidopsis thaliana, Protein phosphorylation, Phosphorylation, Cells, Cultured, biology, Arabidopsis Proteins, Phosphorus, Phosphoproteomics, Biological Transport, Cell Biology, Phosphate, biology.organism_classification, Phosphoproteins, Carbon, 030104 developmental biology, chemistry, Biochemistry, Starvation response, 010606 plant biology & botany
Abstract

Phosphorus absorbed in the form of phosphate (H2 PO4 - ) is an essential but limiting macronutrient for plant growth and agricultural productivity. A comprehensive understanding of how plants respond to phosphate starvation is essential for the development of more phosphate-efficient crops. Here we employed label-free proteomics and phosphoproteomics to quantify protein-level responses to 48 h of phosphate versus phosphite (H2 PO3 - ) resupply to phosphate-deprived Arabidopsis thaliana suspension cells. Phosphite is similarly sensed, taken up and transported by plant cells as phosphate, but cannot be metabolized or used as a nutrient. Phosphite is thus a useful tool for differentiating between non-specific processes related to phosphate sensing and transport and specific responses to phosphorus nutrition. We found that responses to phosphate versus phosphite resupply occurred mainly at the level of protein phosphorylation, complemented by limited changes in protein abundance, primarily in protein translation, phosphate transport and scavenging, and central metabolism proteins. Altered phosphorylation of proteins involved in core processes such as translation, RNA splicing and kinase signaling was especially important. We also found differential phosphorylation in response to phosphate and phosphite in 69 proteins, including splicing factors, translation factors, the PHT1;4 phosphate transporter and the HAT1 histone acetyltransferase - potential phospho-switches signaling changes in phosphorus nutrition. Our study illuminates several new aspects of the phosphate starvation response and identifies important targets for further investigation and potential crop improvement.

Published
2020

27. Phosphate and phosphite differentially impact the proteome and phosphoproteome of Arabidopsis suspension cell cultures

Author

R. Glen Uhrig, William C. Plaxton, Mina Ghahremani, María Pérez-Fernández, Devang Mehta, Maryalle Tan, and Pascal Schläpfer

Subjects
biology, Kinase, Phosphorus, Phosphoproteomics, chemistry.chemical_element, Phosphate, biology.organism_classification, chemistry.chemical_compound, Biochemistry, chemistry, Arabidopsis, Phosphorylation, Arabidopsis thaliana, Protein phosphorylation
Abstract

SUMMARYPhosphorus absorbed in the form of phosphate (H2PO4−) is an essential but limiting macronutrient for plant growth and agricultural productivity. A comprehensive understanding of how plants respond to phosphate starvation is essential to develop more phosphate-efficient crops. Here we employed label-free proteomics and phosphoproteomics to quantify protein-level responses to 48 h of phosphate versus phosphite (H2PO3−) resupply to phosphate-deprived Arabidopsis thaliana suspension cells. Phosphite is similarly sensed, taken up, and transported by plant cells as phosphate, but cannot be metabolized or used as a nutrient. Phosphite is thus a useful tool to delineate between non-specific processes related to phosphate sensing and transport, and specific responses to phosphorus nutrition. We found that responses to phosphate versus phosphite resupply occurred mainly at the level of protein phosphorylation, complemented by limited changes in protein abundance, primarily in protein translation, phosphate transport and scavenging, and central metabolism proteins. Altered phosphorylation of proteins involved in core processes such as translation, RNA splicing, and kinase signalling were especially important. We also found differential phosphorylation in response to phosphate and phosphite in 69 proteins, including splicing factors, translation factors, the PHT1;4 phosphate transporter and the HAT1 histone acetyltransferase—potential phospho-switches signalling changes in phosphorus nutrition. Our study illuminates several new aspects of the phosphate-starvation response and identifies important targets for further investigation and potential crop improvement.

Published
2020
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28. Mitigating the impact of conference and travel cancellations on researchers’ futures

Author

Hedyeh Ebrahimi, Florencia Fernandez-Chiappe, Yaw Bediako, Sarvenaz Sarabipour, Vinodh Ilangovan, Tracey L. Weissgerber, Devang Mehta, Carolina P. Quezada, Andy Tay, Shyam M Saladi, Julia L. Riley, and Charlotte M. de Winde

Subjects
medicine.medical_specialty, Coronavirus disease 2019 (COVID-19), QH301-705.5, Science, Interprofessional Relations, Control (management), Pneumonia, Viral, General Biochemistry, Genetics and Molecular Biology, conferences, Betacoronavirus, science funding, Research Support as Topic, medicine, Humans, Biology (General), Point of View, Pandemics, early-career researchers, Publishing, Internet, Travel, General Immunology and Microbiology, business.industry, Unintended consequences, SARS-CoV-2, General Neuroscience, Public health, Feature Article, COVID-19, General Medicine, Public relations, Congresses as Topic, research assessment, Research Personnel, Career Mobility, Scale (social sciences), Medicine, The Internet, Business, travel, Public Health, Coronavirus Infections, Futures contract, Editorial Policies
Abstract

The need to protect public health during the current COVID-19 pandemic has necessitated conference cancellations on an unprecedented scale. As the scientific community adapts to new working conditions, it is important to recognize that some of our actions may disproportionately affect early-career researchers and scientists from countries with limited research funding. We encourage all conference organizers, funders and institutions who are able to do so to consider how they can mitigate the unintended consequences of conference and travel cancellations and we provide seven recommendations for how this could be achieved. The proposed solutions may also offer long-term benefits for those who normally cannot attend conferences, and thus lead to a more equitable future for generations of researchers.

Published
2020

29. Towards responsible communication of agricultural biotechnology research for the common good

Author

Devang Mehta and Hervé Vanderschuren

Subjects
0303 health sciences, business.industry, Global South, Cell Biology, Agricultural biotechnology, Pipeline (software), 03 medical and health sciences, 0302 clinical medicine, Agriculture, Public trust, Critical assessment, Business, Molecular Biology, Environmental planning, 030217 neurology & neurosurgery, 030304 developmental biology
Abstract

Lack of critical assessment and responsible reporting of proof-of-concept agricultural biotechnologies such as CRISPR–Cas can delay innovation, jeopardize public trust and waste resources, especially in the Global South. In this commentary, we propose solutions to facilitate a more responsible innovation pipeline and to realize the potential of biotechnology in agriculture. Mehta and Vanderschuren advocate for more stringent standards in reporting agricultural biotechnology research.

Published
2021
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30. Genome-scale analysis of regulatory protein acetylation enzymes from photosynthetic eukaryotes

Author

Devang Mehta, R. Glen Uhrig, Wilhelm Gruissem, Matthias Hirsch-Hoffmann, and Pascal Schläpfer

Subjects
0301 basic medicine, Lysine Acetyltransferases, Protein Acetylation, lcsh:QH426-470, lcsh:Biotechnology, Protein domain, Biology, Proteomics, Genome, Evolution, Molecular, 03 medical and health sciences, lcsh:TP248.13-248.65, Genetics, Protein phosphorylation, Amino Acid Sequence, Photosynthesis, Lysine Deacetylase, Phylogeny, Regulation of gene expression, Photosynthetic eukaryotes, Eukaryota, Acetylation, Genomics, Plants, biology.organism_classification, Post-translational modifications, Lysine Acetyltransferase, lcsh:Genetics, 030104 developmental biology, Eukaryote, Protein Processing, Post-Translational, Sequence Alignment, Biotechnology, Research Article, Transcription Factors
Abstract

Background Reversible protein acetylation occurring on Lys-Ne has emerged as a key regulatory post-translational modification in eukaryotes. It is mediated by two groups of enzymes: lysine acetyltransferases (KATs) and lysine deacetylases (KDACs) that catalyze the addition and removal of acetyl groups from target proteins. Estimates indicate that protein acetylation is second to protein phosphorylation in abundance, with thousands of acetylated sites now identified in different subcellular compartments. Considering the important regulatory role of protein phosphorylation, elucidating the diversity of KATs and KDACs across photosynthetic eukaryotes is essential in furthering our understanding of the impact of reversible protein acetylation on plant cell processes. Results We report a genome-scale analysis of lysine acetyltransferase (KAT)- and lysine deacetylase (KDAC)-families from 53 photosynthetic eukaryotes. KAT and KDAC orthologs were identified in sequenced genomes ranging from glaucophytes and algae to land plants and then analyzed for evolutionary relationships. Based on consensus molecular phylogenetic and subcellular localization data we found new sub-classes of enzymes in established KAT- and KDAC-families. Specifically, we identified a non-photosynthetic origin of the HD-tuin family KDACs, a new monocot-specific Class I HDA-family sub-class, and a phylogenetically distinct Class II algal/heterokont sub-class which maintains an ankyrin domain not conserved in land plant Class II KDACs. Protein structure analysis showed that HDA- and SRT-KDACs exist as bare catalytic subunits with highly conserved median protein length, while all KATs maintained auxiliary domains, with CBP- and TAFII250-KATs displaying protein domain gain and loss over the course of photosynthetic eukaryote evolution in addition to variable protein length. Lastly, promoter element enrichment analyses across species revealed conserved cis-regulatory sequences that support KAT and KDAC involvement in the regulation of plant development, cold/drought stress response, as well as cellular processes such as the circadian clock. Conclusions Our results reveal new evolutionary, structural, and biological insights into the KAT- and KDAC-families of photosynthetic eukaryotes, including evolutionary parallels to protein kinases and protein phosphatases. Further, we provide a comprehensive annotation framework through our extensive phylogenetic analysis, from which future research investigating aspects of protein acetylation in plants can use to position new findings in a broader context., BMC Genomics, 18, ISSN:1471-2164

Published
2017
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31. A new full-length circular DNA sequencing method for viral-sized genomes reveals that RNAi transgenic plants provoke a shift in geminivirus populations in the field

Author

Andrea Patrignani, Wilhelm Gruissem, Matthias Hirsch-Hoffmann, Devang Mehta, Hervé Vanderschuren, Mariam Were, Hassan Karakacha Were, Syed Shan-e-Ali Zaidi, and University of Zurich

Subjects
Biochemistry & Molecular Biology, Sequence analysis, VIRUSES, 610 Medicine & health, 10071 Functional Genomics Center Zurich, Computational biology, Genome, Viral, ERRORS, Genome, Virus, law.invention, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, AGE, 1311 Genetics, law, Genetics, Geminiviridae, Polymerase chain reaction, 030304 developmental biology, 0303 health sciences, Science & Technology, biology, Massively Parallel (Deep) Sequencing, POLYMERASE, fungi, High-Throughput Nucleotide Sequencing, Sequence Analysis, DNA, biology.organism_classification, Plants, Genetically Modified, RNA silencing, chemistry, DNA, Viral, Methods Online, 570 Life sciences, RNA Interference, DNA, Circular, Life Sciences & Biomedicine, 030217 neurology & neurosurgery, DNA, Algorithms, Single molecule real time sequencing
Abstract

We present a new method, CIDER-Seq (Circular DNA Enrichment sequencing) for the unbiased enrichment and long-read sequencing of viral-sized circular DNA molecules. We used CIDER-Seq to produce single-read full-length virus genomes for the first time. CIDER-Seq combines PCR-free virus enrichment with Single Molecule Real Time sequencing and a new sequence de-concatenation algorithm. We apply our technique to produce >1200 full-length, highly accurate geminivirus genomes from RNAi-transgenic and control plants in a field trial in Kenya. Using CIDER-Seq we can demonstrate for the first time that the expression of antiviral double-stranded RNA (dsRNA) in transgenic plants causes a consistent shift in virus populations towards species sharing low homology to the transgene derived dsRNA. Our method and its application in an economically important crop plant opens new possibilities in periodic virus sequence surveillance and accurate profiling of diverse circular DNA elements., Nucleic Acids Research, 47 (2), ISSN:1362-4962, ISSN:0301-5610

Published
2019
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32. Highlight negative results to improve science

Author

Devang Mehta

Subjects
0301 basic medicine, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, Multidisciplinary, Publishing, business.industry, MEDLINE, 030206 dentistry, Public relations, business, Psychology, Preference
Abstract

Publishers, reviewers and other members of the scientific community must fight science’s preference for positive results — for the benefit of all, says Devang Mehta. Publishers, reviewers and other members of the scientific community must fight science’s preference for positive results — for the benefit of all, says Devang Mehta.

Published
2019
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33. Full-length sequencing of circular DNA viruses and extrachromosomal circular DNA using CIDER-Seq

Author

Devang, Mehta, Luc, Cornet, Matthias, Hirsch-Hoffmann, Syed Shan-E-Ali, Zaidi, and Hervé, Vanderschuren

Subjects
DNA, Viral, Arabidopsis, Sequence Analysis, DNA, DNA, Circular, Nucleic Acid Amplification Techniques
Abstract

Circular DNA is ubiquitous in nature in the form of plasmids, circular DNA viruses, and extrachromosomal circular DNA (eccDNA) in eukaryotes. Sequencing of such molecules is essential to profiling virus distributions, discovering new viruses and understanding the roles of eccDNAs in eukaryotic cells. Circular DNA enrichment sequencing (CIDER-Seq) is a technique to enrich and accurately sequence circular DNA without the need for polymerase chain reaction amplification, cloning, and computational sequence assembly. The approach is based on randomly primed circular DNA amplification, which is followed by several enzymatic DNA repair steps and then by long-read sequencing. CIDER-Seq includes a custom data analysis package (CIDER-Seq Data Analysis Software 2) that implements the DeConcat algorithm to deconcatenate the long sequencing products of random circular DNA amplification into the intact sequences of the input circular DNA. The CIDER-Seq data analysis package can generate full-length annotated virus genomes, as well as circular DNA sequences of novel viruses. Applications of CIDER-Seq also include profiling of eccDNA molecules such as transposable elements (TEs) from biological samples. The method takes ~2 weeks to complete, depending on the computational resources available. Owing to the present constraints of long-read single-molecule sequencing, the accuracy of circular virus and eccDNA sequences generated by the CIDER-Seq method scales with sequence length, and the greatest accuracy is obtained for molecules10 kb long.

Published
2019

34. Additional file 1: of Linking CRISPR-Cas9 interference in cassava to the evolution of editing-resistant geminiviruses

Author

Devang Mehta, Stürchler, Alessandra, Anjanappa, Ravi, Zaidi, Syed, Hirsch-Hoffmann, Matthias, Gruissem, Wilhelm, and Vanderschuren, Hervé

Abstract

Table S1. Virus infection results (confirmation experiment). Table S2. Proportion of ACMV-AC2 H54Q viruses detected by deep-sequencing in N. benthamiana. Table S3. Primer sequences. Table S4. Sequencing Barcodes. Figure S1. Analysis of virus sequences from infected plants at (a) 3 and (b) 8 weeks post infection. Figure S2. Analysis of viral proteins from edited and control populations obtained by single molecule amplicon sequencing at 3 weeks post infection. Figure S3. Analysis of viral proteins from edited and control populations obtained by single molecule amplicon sequencing at 8 weeks post infection. Figure S4. In vitro cleavage assay of the ACMV-AC2 H54Q mutant. Figure S5. Southern blot analysis for number of T-DNA integration events per plant line. * Figure S6. (a) Western blots for Cas9-GFP expression. (b) Raw blot images acquired using an Odyssey CLX imager for anti-Cas9 and anti-Actin probing of protein extracts from Cas9+sgRNA1 lines. (c) Raw blot images for probing Cas9 lines protein extracts with anti-Cas9 and anti-Actin antibodies. Figure S7. Symptom scoring scale. Figure S8. Analysis of full-length virus sequences from infected plants at 8 weeks post infection. (DOCX 6747 kb)

Published
2019
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36. The Green Revolution did not increase poverty and hunger for millions

Author

Devang Mehta

Subjects
0106 biological sciences, Poverty, business.industry, Hunger, 04 agricultural and veterinary sciences, Plant Science, 01 natural sciences, The arts, Agricultural economics, Crop Production, Plant Breeding, Geography, Crop production, Agriculture, 040103 agronomy & agriculture, 0401 agriculture, forestry, and fisheries, Humans, Plant breeding, business, Green Revolution, 010606 plant biology & botany
Published
2018

37. Molecular insights into Cassava brown streak virus susceptibility and resistance by profiling of the early host response

Author

Hervé Vanderschuren, Wilhelm Gruissem, Alicja Szabelska, Ravi B. Anjanappa, Devang Mehta, Michal J. Okoniewski, University of Zurich, and Vanderschuren, Hervé

Subjects
0301 basic medicine, Manihot, salicylic acid, Soil Science, RNA-Seq, 610 Medicine & health, 10071 Functional Genomics Center Zurich, Plant Science, Plasmodesma, Plant disease resistance, Biology, cassava, Transcriptome, 03 medical and health sciences, chemistry.chemical_compound, Plant virus, 1110 Plant Science, 1312 Molecular Biology, 1102 Agronomy and Crop Science, Molecular Biology, Gene, Glucans, 1111 Soil Science, Plant Diseases, Genetics, RDR1, Callose, food and beverages, Original Articles, Potyviridae, 3. Good health, RNA silencing, 030104 developmental biology, chemistry, ipomovirus, virus resistance, callose, CBSV, RNA- seq, RNA‐seq, 570 Life sciences, biology, Original Article, Agronomy and Crop Science
Abstract

Cassava brown streak virus (CBSV) and Ugandan cassava brown streak virus (UCBSV) are responsible for significant cassava yield losses in eastern sub-Saharan Africa. To study the possible mechanisms of plant resistance to CBSVs, we inoculated CBSV-susceptible and CBSV-resistant cassava varieties with a mixed infection of CBSVs using top-cleft grafting. Transcriptome profiling of the two cassava varieties was performed at the earliest time point of full infection (28 days after grafting) in the susceptible scions. The expression of genes encoding proteins in RNA silencing, salicylic acid pathways and callose deposition was altered in the susceptible cassava variety, but transcriptional changes were limited in the resistant variety. In total, the expression of 585 genes was altered in the resistant variety and 1292 in the susceptible variety. Transcriptional changes led to the activation of β-1,3-glucanase enzymatic activity and a reduction in callose deposition in the susceptible cassava variety. Time course analysis also showed that CBSV replication in susceptible cassava induced a strong up-regulation of RDR1, a gene previously reported to be a susceptibility factor in other potyvirus–host pathosystems. The differences in the transcriptional responses to CBSV infection indicated that susceptibility involves the restriction of callose deposition at plasmodesmata. Aniline blue staining of callose deposits also indicated that the resistant variety displays a moderate, but significant, increase in callose deposition at the plasmodesmata. Transcriptome data suggested that resistance does not involve typical antiviral defence responses (i.e. RNA silencing and salicylic acid). A meta-analysis of the current RNA-sequencing (RNA-seq) dataset and selected potyvirus–host and virus–cassava RNA-seq datasets revealed that the conservation of the host response across pathosystems is restricted to genes involved in developmental processes. ISSN:1464-6722 ISSN:1364-3703

Published
2018
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38. CRISPR-Cas9 interference in cassava linked to the evolution of editing-resistant geminiviruses

Author

Matthias Hirsch-Hoffmann, Alessandra Sturchler, Hervé Vanderschuren, Devang Mehta, and Wilhelm Gruissem

Subjects
0106 biological sciences, Genetics, 0303 health sciences, biology, viruses, food and beverages, biology.organism_classification, Plant biology, 01 natural sciences, Genome, Virus, 03 medical and health sciences, chemistry.chemical_compound, chemistry, African cassava mosaic virus, CRISPR, DNA, 030304 developmental biology, 010606 plant biology & botany
Abstract

We used CRISPR-Cas9 in the staple food crop cassava with the aim of engineering resistance to African cassava mosaic virus, a member of a widespread and important family of plant-pathogenic DNA viruses. We found that between 33 and 48% of edited virus genomes evolved a conserved single-nucleotide mutation that confers resistance to CRISPR-Cas9 cleavage. Our study highlights the potential for virus escape from this technology. Care should be taken to design CRISPR-Cas9 experiments that minimize the risk of virus escape.

Published
2018
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39. Accelerated ex situ breeding of

Author

Simon E, Bull, David, Seung, Christelle, Chanez, Devang, Mehta, Joel-Elias, Kuon, Elisabeth, Truernit, Anton, Hochmuth, Irene, Zurkirchen, Samuel C, Zeeman, Wilhelm, Gruissem, and Hervé, Vanderschuren

Subjects
Crops, Agricultural, Gene Editing, Manihot, Arabidopsis Proteins, fungi, Plant Sciences, food and beverages, SciAdv r-articles, Germination, Starch, Plants, Genetically Modified, Plant Breeding, Starch Synthase, Mutagenesis, CRISPR-Cas Systems, Molecular Biology, Research Articles, Plant Proteins, Research Article
Abstract

The growing need for cassava, a food and fuel crop, has led to a new plant breeding technique designed to accelerate breeding of cassava with modified starch., Crop diversification required to meet demands for food security and industrial use is often challenged by breeding time and amenability of varieties to genome modification. Cassava is one such crop. Grown for its large starch-rich storage roots, it serves as a staple food and a commodity in the multibillion-dollar starch industry. Starch is composed of the glucose polymers amylopectin and amylose, with the latter strongly influencing the physicochemical properties of starch during cooking and processing. We demonstrate that CRISPR-Cas9 (clustered regularly interspaced short palindromic repeats/CRISPR-associated protein 9)–mediated targeted mutagenesis of two genes involved in amylose biosynthesis, PROTEIN TARGETING TO STARCH (PTST1) or GRANULE BOUND STARCH SYNTHASE (GBSS), can reduce or eliminate amylose content in root starch. Integration of the Arabidopsis FLOWERING LOCUS T gene in the genome-editing cassette allowed us to accelerate flowering—an event seldom seen under glasshouse conditions. Germinated seeds yielded S1, a transgene-free progeny that inherited edited genes. This attractive new plant breeding technique for modified cassava could be extended to other crops to provide a suite of novel varieties with useful traits for food and industrial applications.

Published
2018

40. A new full-length virus genome sequencing method reveals that antiviral RNAi changes geminivirus populations in field-grown cassava

Author

Hervé Vanderschuren, Matthias Hirsch-Hoffmann, Andrea Patrignani, Wilhelm Gruissem, Mariam Were, Devang Mehta, and Hassan Karakacha Were

Subjects
0106 biological sciences, Transposable element, 0303 health sciences, Sequence assembly, Genomics, Computational biology, Biology, 01 natural sciences, Genome, Virus, DNA sequencing, 03 medical and health sciences, Plasmid, 030304 developmental biology, 010606 plant biology & botany, Single molecule real time sequencing
Abstract

Deep-sequencing of virus isolates using short-read sequencing technologies is problematic since viruses are often present in complexes sharing a high-degree of sequence identity. The full-length genomes of such highly-similar viruses cannot be assembled accurately from short sequencing reads. We present a new method, CIDER-Seq (Circular DNA Enrichment Sequencing) which successfully generates accurate full-length virus genomes from individual sequencing reads with no sequence assembly required. CIDER-Seq operates by combining a PCR-free, circular DNA enrichment protocol with Single Molecule Real Time sequencing and a new sequence deconcatenation algorithm. We apply our technique to produce more than 1,200 full-length, highly accurate geminivirus genomes from RNAi-transgenic and control plants in a field trial in Kenya. Using CIDER-Seq we can demonstrate for the first time that the expression of antiviral doublestranded RNA (dsRNA) in transgenic plants causes a consistent shift in virus populations towards species sharing low homology to the transgene derived dsRNA. Our results show that CIDER-seq is a powerful, cost-effective tool for accurately sequencing circular DNA viruses, with future applications in deep-sequencing other forms of circular DNA such as transposons and plasmids.

Published
2017
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43. PhD supervisors: be better mentors

Author

Konstantinos Vavitsas and Devang Mehta

Subjects
0301 basic medicine, Medical education, Multidisciplinary, business.industry, Mentors, Mentoring, Europe, 03 medical and health sciences, Leadership, 030104 developmental biology, Text mining, Mental Health, Humans, Synthetic Biology, Sociology, Education, Graduate, business, Students
Published
2017

44. Early transcriptome analysis of the brown streak virus–cassava pathosystem provides molecular insights into virus susceptibility and resistance

Author

Ravi B. Anjanappa, Hervé Vanderschuren, Wilhelm Gruissem, Michal J. Okoniewski, Alicja Szabelska, and Devang Mehta

Subjects
0106 biological sciences, 0303 health sciences, Host (biology), Callose, food and beverages, Plasmodesma, Biology, 01 natural sciences, Virus, Microbiology, Transcriptome, 03 medical and health sciences, RNA silencing, chemistry.chemical_compound, Pathosystem, chemistry, Gene, 030304 developmental biology, 010606 plant biology & botany
Abstract

SUMMARYCassava brown streak viruses (CBSVs) are responsible for significant cassava yield losses in eastern sub–Saharan Africa. In the present work, we inoculated CBSV–susceptible and –resistant cassava varieties with a mixed infection of CBSVs using top-cleft grafting. Virus titres in grafted scions were monitored in a time course experiment in both varieties. We performed RNA-seq of the two cassava varieties at the earliest time-point of full infection in the susceptible scions. Genes encoding proteins in RNA silencing and salicylic acid pathways were regulated in the susceptible cassava variety but transcriptional changes were limited in the resistant variety. After infection, genes related to callose deposition at plasmodesmata were regulated and callose deposition was significantly reduced in the susceptible cassava variety. We also show that β–1,3–glucanase enzymatic activity is differentially regulated in the susceptible and resistant varieties. The differences in transcriptional responses to CBSV infection indicate that resistance involves callose deposition at plasmodesmata but does not trigger typical anti-viral defence responses. A meta-analysis of the current RNA-seq dataset and selected, previously reported, host–potyvirus and virus-cassava RNA-seq datasets revealed comparable host responses across pathosystems only at similar time points after infection or infection of a common host.HIGHLIGHTOur results suggest that resistance to CBSV in cassava involves callose deposition at the plasmodesmata and our meta-analysis of multiple virus-crop RNA-seq studies suggests that conserved responses across different host-virus systems are limited and depend greatly on time after infection.

Published
2017
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46. Characterization of brown streak virus-resistant cassava

Author

Wilhelm Gruissem, Ravi B. Anjanappa, Devang Mehta, Edward Kanju, Hervé Vanderschuren, and Midatharahally N. Maruthi

Subjects
0301 basic medicine, Veterinary medicine, Manihot, S1, Physiology, Cassava brown streak virus, Streak, Virus, Crop, 03 medical and health sciences, Cultivar, Disease Resistance, Plant Diseases, 2. Zero hunger, Ugandan cassava brown streak virus, biology, Inoculation, food and beverages, General Medicine, Potyviridae, Viral Load, biology.organism_classification, Virology, 030104 developmental biology, Agronomy and Crop Science, Mixed infection
Abstract

Cassava brown streak disease (CBSD) has become a major constraint to cassava production in East and Central Africa. The identification of new sources of CBSD resistance is essential to deploy CBSD mitigation strategies as the disease is progressing westwards to new geographical areas. A stringent infection method based on top cleft grafting combined with precise virus titer quantitation was utilized to screen fourteen cassava cultivars and elite breeding lines. When inoculated with mixed infections of Cassava brown streak virus (CBSV) and Ugandan cassava brown streak virus (UCBSV), the scions of elite breeding lines KBH 2006/18 and KBH 2006/26 remained symptom-free during a 16-week period of virus graft inoculation, while susceptible varieties displayed typical CBSD infection symptoms at 4 weeks after grafting. The identified CBSD resistance was stable under the co-inoculation of CBSV, UCBSV with cassava geminiviruses (CGMs). Double grafting experiments revealed that transmission of CBSV and UCBSV to CBSD susceptible top scions was delayed when using intermediate scions of elite breeding lines KBH 2006/18 and KBH 2006/26. Nonetheless, comparison of virus systemic movement using scions from KBH2006/18 and a transgenic CBSD resistant 60444 line (60444-Hp9 line) showed that both CBSV and UCBSV move at undetectable levels through the stems. Further, protoplast-based assays of virus titers over time showed that the replication of CBSVs is inhibited in the resistant line KBH2006/18, suggesting that the identified CBSD resistance is at least partially based on inhibition of virus replication. Our molecular characterization of CBSD resistance in cassava offers a robust virus–host system to further investigate the molecular determinants of CBSD resistance.

Published
2016

47. Lab heads should learn to talk about racism

Author

Devang Mehta

Subjects
0301 basic medicine, 03 medical and health sciences, 030104 developmental biology, Multidisciplinary, business.industry, media_common.quotation_subject, Sociology, Public relations, business, Racism, media_common
Abstract

Senior academics must step up and take the lead in discussing intolerance, says Devang Mehta. Senior academics must step up and take the lead in discussing intolerance, says Devang Mehta.

Published
2018
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48. Binary Systems of Mesogens and Non-mesogens exhibiting Mesomorphism

Author

R. A VORA, RENU GUPTA, and DEVANG MEHTA

Subjects
Mesomorphism, Smectic, Mesogens
Abstract

Applied Chemistry Department, faculty of Technology & Engineering, M. S. University of Baroda, Baroda-390 001 Manuscript received 29 December 1992, accepted 9 March 1993 Liquid crystal formation in eight binary systems are reported in which one or both the components are non-mesogens. The binary systems of non-mesogens, comprising of components with terminal nitro or chloro substituent, exhibit induced smectic or nematic mesophases; induction of mesophase is higher in magnitude for a nitro group as compared to a chloro group. Shorter alkyl/alkoxy chains are not conducive to the mixed mesomorphism, probably due to lack of marked depression in melting points. The systems incorporating a monotropic mesogen and a non-mesogen, exhibit mesomorphic properties comparable with the binary systems of non-mesogens of the present work. Some of the binary compositions exhibit smectic phase at ambient temperature on cooling. The latent transition temperatures for non-mesogens are obtained and the phase diagrams are discussed in detail.

Published
1993
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49. Accelerated ex situ breeding of GBSS - and PTST1 -edited cassava for modified starch

Author

Irene Zurkirchen, Hervé Vanderschuren, David Seung, Anton Hochmuth, Christelle Chanez, Simon E. Bull, Wilhelm Gruissem, Samuel C. Zeeman, Joel‑Elias Kuon, Elisabeth Truernit, and Devang Mehta

Subjects
0301 basic medicine, Starch, Locus (genetics), Biology, Modified starch, Crop, 03 medical and health sciences, chemistry.chemical_compound, Amylose, Arabidopsis, AMYLOSE-FREE STARCH, PASTING PROPERTIES, TOOL, Plant breeding, Food science, GENE-EXPRESSION, 2. Zero hunger, Multidisciplinary, Science & Technology, GELATINIZATION, CROP, food and beverages, DNA, biology.organism_classification, ARABIDOPSIS, WAXY, Multidisciplinary Sciences, 030104 developmental biology, chemistry, Amylopectin, Science & Technology - Other Topics, RNA
Abstract

Crop diversification required to meet demands for food security and industrial use is often challenged by breeding time and amenability of varieties to genome modification. Cassava is one such crop. Grown for its large starch-rich storage roots, it serves as a staple food and a commodity in the multibillion-dollar starch industry. Starch is composed of the glucose polymers amylopectin and amylose, with the latter strongly influencing the physicochemical properties of starch during cooking and processing. We demonstrate that CRISPR-Cas9 (clustered regularly interspaced short palindromic repeats/CRISPR-associated protein 9)-mediated targeted mutagenesis of two genes involved in amylose biosynthesis, PROTEIN TARGETING TO STARCH (PTST1) or GRANULE BOUND STARCH SYNTHASE (GBSS), can reduce or eliminate amylose content in root starch. Integration of the Arabidopsis FLOWERING LOCUS T gene in the genome-editing cassette allowed us to accelerate flowering-an event seldom seen under glasshouse conditions. Germinated seeds yielded S1, a transgene-free progeny that inherited edited genes. This attractive new plant breeding technique for modified cassava could be extended to other crops to provide a suite of novel varieties with useful traits for food and industrial applications. ispartof: Science Advances vol:4 issue:9 ispartof: location:United States status: published

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