Carbon metabolism in transgenic roots with altered levels of hexokinase and triosephosphate isomerase and growing under different nitrogen status

Sedaghatkish, Afsaneh

01 1900

Ce projet a pour but d’évaluer la capacité de la voie des pentoses phosphates (VPP) dans les racines transgéniques de pomme de terre (Solanum tuberosum) modifiées pour exprimer différents niveaux de l'hexokinase (HK) et de la triosephosphate isomérase cytosolique (cTPI). Dans les racines, la VPP alimente la voie de l’assimilation de l’azote en equivalents réducteurs et permet donc la biosynthèse des acides aminés. Le glucose-6-phosphate produit par l’HK est consommé par la partie oxydative de la VPP catalysée par la glucose-6-phosphate déshydrogénase (G6PDH) et la 6-phosphogluconate déshydrogénase (6PGDH). Les changements dans l'expression de HK et cTPI peuvent affecter le fonctionnement de la VPP et les mécanismes qui sont liés à l’utilisation des équivalents réducteurs produits par la VPP, comme l'assimilation de l’azote et la synthèse des acides aminés. Afin d’évaluer l’effet des manipulations génétiques de l’HK et de la cTPI sur l’assimilation de l’azote, nous avons cultivé les racines transgéniques sur des milieux contenant des concentrations élevées (7 mM) ou basses (0,7 mM) de nitrate d’ammonium comme source d’azote. Les résultats montrent que la culture sur un milieu riche en azote induit les activités G6PDH et 6PGDH. Les données montrent que la capacité de la VPP est plus grande avec des niveaux élevés en HK ou en cTPI. Nous avons aussi pu démontrer une plus grande activité spécifique de l’HK dans les conditions pauvres en azote. Ces données ont été complémentées par des mesures des pools d’acides aminés dans les racines transgéniques cultivées sur différents niveaux d’azote. Aucune tendance notable des pools d’acides aminés n’a été remarquée dans les racines modifiées pour leur contenu en HK suggèrant que la manipulation de HK n’affecte pas l'assimilation de l’azote. Dans les racines transgéniques modifiées pour la cTPI, les ratios Gln/Glu et Asn/Asp sont plus élevés chez les clones antisens, indiquant une assimilation de l’azote plus élevée. Ces résultats ont démontré l'activation de l'assimilation de l’azote chez les clones antisens cTPI dans les conditions élevées et basses d’azote alors que la manipulation de l’HK n’affecte pas l’assimilation de l’azote. / This study investigates the capacity of the oxidative pentose phosphate pathway (oxPPP) and nitrogen metabolism in transgenic potato (Solanum tuberosum) roots modified to express different levels of hexokinase (HK) or cytosolic triosephosphate isomerase (cTPI) growing under different nitrogen regimes. The flux of carbon through the oxPPP in cTPI antisense roots is higher than control roots growing under high supply of N. On the other hand, the conversion of Glucose (Glc) to Glucose-6-phosphate (G6P) is higher in roots overexpressing HK than in antisense HK roots growing at a high level of N. Therefore, overexpression of HK or down regulation of cTPI activities in transgenic roots might be compensated by increased C catabolism through the oxPPP. In order to see the affect of HK and cTPI manipulation on N assimilation, the transgenic roots were grown on media with low or high concentration of ammonium nitrate as the N source. The specific activity of the oxPPP enzymes glucose-6-phosphate dehydrogenase (G6PDH) and 6-phosphogluconate dehydrogenase (6PGDH) were both increased by an increased N supply in HK and cTPI transgenic roots. This is consistent with the provision of reducing equivalents for N assimilation. The data also show that the capacity of the oxPPP is higher in roots with high HK or cTPI activity. We were able to detect higher HK specific activity in N deficient conditions. These data were complemented with measurements of amino acid pools in transgenic roots. No trend in amino acid pools was found in roots modified for HK activity. However, down regulation of cTPI led to higher Gln, Gln/Glu and Asn/Asp ratios, indicating higher assimilation of N. These results demonstrated the activation of N assimilation in cTPI antisense clones while the manipulation of HK is unlikely to affect the N assimilation.

Hexokinase

Triosephosphate isomérase

Acides aminés

Nutrition azotée

Voie des pentoses phosphates

Triosephosphate isomerase

Nitrogen assimilation

Oxidative pentose phosphate pathway

Amino acid content

ORGAN-SPECIFIC EPIGENOMIC AND TRANSCRIPTOMIC CHANGES IN RESPONSE TO NITRATE IN TOMATO

Russell S Julian (8810357)

21 June 2022

Nitrogen (N), an essential plant macronutrient, is among the most limiting factors of crop yield. To sustain modern agriculture, N is often amended in soil in the form of chemical N fertilizer, a major anthropogenic contributor to nutrient pollution that affects climate, biodiversity and human health. To achieve agricultural sustainability, a comprehensive understanding of the regulation of N response in plants is required, in order to engineer crops with higher N use efficiency. Recently, epigenetic mechanisms, such as histone modifications, have gained increasing importance as a new layer of regulation of biological processes. However, our understanding of how epigenetic processes regulate N uptake and assimilation is still in its infancy. To fill this knowledge gap, we first performed a meta-analysis that combined functional genomics and network inference approaches to identify a set of N-responsive epigenetic regulators and predict their effects in regulating epigenome and transcriptome during plant N response. Our analysis suggested that histone modifications could serve as a regulatory mechanism underlying the global transcriptomic reprogramming during plant N response. To test this hypothesis, I applied chromatin immunoprecipitation-sequencing (ChIP-Seq) to monitor the genome-wide changes of four histone marks (H3K27ac, H3K4me3, H3K36me3 and H3K27me3) in response to N supply in tomato plants, followed by RNA-Seq to profile the transcriptomic changes. To investigate the organ specificity of histone modifications, I assayed shoots and roots separately. My results suggest that up to two-thirds of differentially expressed genes (DEGs) are modified in at least one of the four histone marks, supporting an integral role of histone modification in regulating N response. I observed a synergistic modification of active histone marks (H3K27ac, H3K4me3 and H3K36me3) at gene loci functionally relevant to N uptake and assimilation. Surprisingly, I uncovered a non-canonical role of H3K27me3, which is conventionally associated with repressed genes, in modulating active gene expression. Interestingly, such regulatory role of H3K27me3 is specifically associated with highly expressed genes or low expressed genes, depending on the organ context. Overall, I revealed the multi-faceted role of histone marks in mediating the plant N response, which will guide breeding and engineering of better crops with higher N use efficiency

Genomics

Plant cell and molecular biology

Plant physiology

Plant biology not elsewhere classified

Animal cell and molecular biology

epigenetics

epigenomics

nitrogen response

transcriptome analysis

tomato

organ-specific

tomato root

tomato shoot

H3K27me3

H3K4me3

H3K27ac

H3K36me3

INFERNET

nitrogen uptake

nitrogen assimilation

histone marks

ChIP-Seq

RNA-Seq

Botany

Genomics

Molecular Biology

Plant Biology

Plant Cell and Molecular Biology

Plant Physiology