Pooled <scp>CRISPR</scp>/Cas9 reveals redundant roles of plastidial phosphoglycerate kinases in carbon fixation and metabolism

Li, Rui-Zi; Qiu, Zhimin; Wang, Xiaoguo; Gong, Pingping; Xu, Qinzhen; Yu, Qing-Bo; Guan, Yuefeng

doi:10.1111/tpj.14303

Cited by 29 publications

(25 citation statements)

References 52 publications

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“…It is very difficult to directly measure the membrane lipid component contents of chloroplasts isolated from maize anthers by thin layer chromatography and gas-liquid chromatography because of the large amounts of very small anther tissues required for chloroplast extraction (Wang and Benning, 2011;Murphy et al, 2015;Block and Albrieux, 2018). Nonetheless, the MGDG, DGDG, and SQDG contents of whole anther tissue estimated by liquid chromatography-mass spectrometry (Ryu and Wang, 1996;Welti et al, 2002) may be used as an indicator of MGDG, DGDG, and SQDG contents in the membranes of anther En chloroplasts, based on similar results reported recently (Chen et al, 2015;Basnet et al, 2019;Li et al, 2019aLi et al, , 2019bLiu et al, 2020). Therefore, liquid chromatography-mass spectrometry provides us with a good opportunity to explore the function of ZmMs33 in anther chloroplast development and function.…”

Section: Loss Of Zmms33 Function Causes H 2 O 2 Accumulation Inmentioning

confidence: 66%

“…For example, Multiple Archesporial Cell 1 (MAC1) , Male Sterile Converted Anther 1 (MSCA1) (Kelliher and Walbot, 2012), Male Sterility 23 (Ms23) (Nan et al, 2017), Ms32 (Moon et al, 2013), and Out Cell Layer 4 (OCL4) (Vernoud et al, 2009) participate in premeiotic morphogenesis, and Abnormal Pollen Vacuolation 1 (APV1) (Somaratne et al, 2017), ZmMs7 (Zhang et al, 2018;An et al, 2020), Irregular Pollen Exine 1 (IPE1)/ZmMs20 (Chen et al, 2017;Wang et al, 2019), Ms26 (Djukanovic et al, 2013), ZmMs30 (An et al, 2019), ZmMs33 (Xie et al, 2018;Zhu et al, 2019), ms44 (Fox et al, 2017), Ms45 (Cigan et al, 2001), and Ms6021 (Tian et al, 2017) are required for anther development and pollen formation during the meiotic and postmeiotic stages in maize. In addition, non-coding RNAs (e.g., miRNAs and ceRNAs) are also involved in maize anther development and pollen formation (Li et al, 2019a(Li et al, , 2019b. Nevertheless, little is known about the metabolic mechanisms that underlie male sterility in maize or about the changes in production, distribution, and utilization of energy and nutrients (e.g., saccharides, lipids, and proteins) that ultimately result in male sterility of GMS mutant anthers.…”

Section: Introductionmentioning

confidence: 99%

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Normal Structure and Function of Endothecium Chloroplasts Maintained by ZmMs33-Mediated Lipid Biosynthesis in Tapetal Cells Are Critical for Anther Development in Maize

Zhu

et al. 2020

Molecular Plant

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Genic male sterility (GMS) is critical for heterosis utilization and hybrid seed production. Although GMS mutants and genes have been studied extensively in plants, it has remained unclear whether chloroplast-associated photosynthetic and metabolic activities are involved in the regulation of anther development. In this study, we characterized the function of ZmMs33/ZmGPAT6, which encodes a member of the glycerol-3-phosphate acyltransferase (GPAT) family that catalyzes the first step of the glycerolipid synthetic pathway. We found that normal structure and function of endothecium (En) chloroplasts maintained by ZmMs33-mediated lipid biosynthesis in tapetal cells are crucial for maize anther development. ZmMs33 is expressed mainly in the tapetum at early anther developmental stages and critical for cell proliferation and expansion at late stages. Chloroplasts in En cells of wild-type anthers function as starch storage sites before stage 10 but as photosynthetic factories since stage 10 to enable starch metabolism and carbohydrate supply. Loss of ZmMs33 function inhibits the biosynthesis of glycolipids and phospholipids, which are major components of En chloroplast membranes, and disrupts the development and function of En chloroplasts, resulting in the formation of abnormal En chloroplasts containing numerous starch granules. Further analyses reveal that starch synthesis during the day and starch degradation at night are greatly suppressed in the mutant anthers, leading to carbon starvation and low energy status, as evidenced by low trehalose-6-phosphate content and a reduced ATP/AMP ratio. The energy sensor and inducer of autophagy, SnRK1, was activated to induce early and excessive autophagy, premature PCD, and metabolic reprogramming in tapetal cells, finally arresting the elongation and development of mutant anthers. Taken together, our results not only show that ZmMs33 is required for normal structure and function of En chloroplasts but also reveal that starch metabolism and photosynthetic activities of En chloroplasts at different developmental stages are essential for normal anther development. These findings provide novel insights for understanding how lipid biosynthesis in the tapetum, the structure and function of En chloroplasts, and energy and substance metabolism are coordinated to maintain maize anther development.

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Section: Loss Of Zmms33 Function Causes H 2 O 2 Accumulation Inmentioning

confidence: 66%

Section: Introductionmentioning

confidence: 99%

Normal Structure and Function of Endothecium Chloroplasts Maintained by ZmMs33-Mediated Lipid Biosynthesis in Tapetal Cells Are Critical for Anther Development in Maize

Zhu

et al. 2020

Molecular Plant

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“…The upregulation of glycolytic enzymes caused by the expression of BnLACS2 in yeast prompted us to then detect whether these genes were altered in BnLACS2 transgenic rapeseed plants. qRT-PCR analysis revealed that the expression of genes for key glycolytic enzymes, including phosphofructokinase (PFK), phosphoglycerate kinase (PGK), enolase (ENO) and pyruvate kinase (PYK) [36][37][38] were significantly increased in BnLACS2-OE transgenic plants, while the expression of those genes were decreased in BnLACS2-RNAi transgenic plants, compared to non-transgenic plants (Fig. 7).…”

Section: Bnlacs2 Overexpression Influences the Expression Of Genes Inmentioning

confidence: 99%

Long-chain acyl-CoA synthetase 2 is involved in seed oil production in Brassica napus

Ding

Zhu

et al. 2020

BMC Plant Biol

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Background: Triacylglycerols (TAGs) are the main composition of plant seed oil. Long-chain acyl-coenzyme A synthetases (LACSs) catalyze the synthesis of long-chain acyl-coenzyme A, which is one of the primary substrates for TAG synthesis. In Arabidopsis, the LACS gene family contains nine members, among which LACS1 and LACS9 have overlapping functions in TAG biosynthesis. However, functional characterization of LACS proteins in rapeseed have been rarely reported. Results: An orthologue of the Arabidopsis LACS2 gene (BnLACS2) that is highly expressed in developing seeds was identified in rapeseed (Brassica napus). The BnLACS2-GFP fusion protein was mainly localized to the endoplasmic reticulum, where TAG biosynthesis occurs. Interestingly, overexpression of the BnLACS2 gene resulted in significantly higher oil contents in transgenic rapeseed plants compared to wild type, while BnLACS2-RNAi transgenic rapeseed plants had decreased oil contents. Furthermore, quantitative real-time PCR expression data revealed that the expression of several genes involved in glycolysis, as well as fatty acid (FA) and lipid biosynthesis, was also affected in transgenic plants. Conclusions: A long chain acyl-CoA synthetase, BnLACS2, located in the endoplasmic reticulum was identified in B. napus. Overexpression of BnLACS2 in yeast and rapeseed could increase oil content, while BnLACS2-RNAi transgenic rapeseed plants exhibited decreased oil content. Furthermore, BnLACS2 transcription increased the expression of genes involved in glycolysis, and FA and lipid synthesis in developing seeds. These results suggested that BnLACS2 is an important factor for seed oil production in B. napus.

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“…For multiplex, more than two sgRNA expression cassettes could be assembled in each of these vectors (Du et al, 2016;Do et al, 2019). Usually, a number of engineered editing reagents for ZFNs, TELENs, or CRISPR/Cas systems, does not show editing activity and cannot create any mutation event in vivo without knowing any cause (Li R. et al, 2019). Therefore, identification of mutations in vivo by validating sgRNA expression and nuclease activity for specific editing reagents via transient assay could save time and resources, and increase success rate before transformation for creating genome edited plants (Do et al, 2019;Bai et al, 2020).…”

Section: Gmu6mentioning

confidence: 99%

“…PCR/RE assay detection method was used frequently in soybean (Michno et al, 2015;Sun et al, 2015;Kanazashi et al, 2018;Di et al, 2019). T7EI assay was occasionally used (Cai et al, 2015;Du et al, 2016) and PCR/Sequencing assay is now the most popular method used to detect mutation in soybean (Haun et al, 2014;Campbell et al, 2019;Cheng et al, 2019;Do et al, 2019;Han et al, 2019;Li R. et al, 2019;Wang J. et al, 2020). PCR/RE and T7EI are cost efficient method when large number putative mutations need to be screened, but limitation of restriction enzyme cut sites can restrict design of sgRNA.…”

Section: Screening Of Mutation Events Created By Ge (Figures 2l-m)mentioning

confidence: 99%

Progresses, Challenges, and Prospects of Genome Editing in Soybean (Glycine max)

Zhang

et al. 2020

Front. Plant Sci.

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Soybean is grown worldwide for oil and protein source as food, feed and industrial raw material for biofuel. Steady increase in soybean production in the past century mainly attributes to genetic mediation including hybridization, mutagenesis and transgenesis. However, genetic resource limitation and intricate social issues in use of transgenic technology impede soybean improvement to meet rapid increases in global demand for soybean products. New approaches in genomics and development of site-specific nucleases (SSNs) based genome editing technologies have expanded soybean genetic variations in its germplasm and have potential to make precise modification of genes controlling the important agronomic traits in an elite background. ZFNs, TALENS and CRISPR/Cas9 have been adapted in soybean improvement for targeted deletions, additions, replacements and corrections in the genome. The availability of reference genome assembly and genomic resources increases feasibility in using current genome editing technologies and their new development. This review summarizes the status of genome editing in soybean improvement and future directions in this field.

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Pooled CRISPR/Cas9 reveals redundant roles of plastidial phosphoglycerate kinases in carbon fixation and metabolism

Cited by 29 publications

References 52 publications

Normal Structure and Function of Endothecium Chloroplasts Maintained by ZmMs33-Mediated Lipid Biosynthesis in Tapetal Cells Are Critical for Anther Development in Maize

Normal Structure and Function of Endothecium Chloroplasts Maintained by ZmMs33-Mediated Lipid Biosynthesis in Tapetal Cells Are Critical for Anther Development in Maize

Long-chain acyl-CoA synthetase 2 is involved in seed oil production in Brassica napus

Progresses, Challenges, and Prospects of Genome Editing in Soybean (Glycine max)

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