Genome-wide analysis of H3K4me3 and H3K27me3 modifications due to Lr28 for leaf rust resistance in bread wheat (Triticum aestivum)

被引:8
作者
Saripalli, Gautam [1 ]
Singh, Kalpana [2 ]
Gautam, Tinku [1 ]
Kumar, Santosh [3 ]
Raghuvanshi, Saurabh [3 ]
Prasad, Pramod [4 ]
Jain, Neelu [5 ]
Sharma, P. K. [1 ]
Balyan, H. S. [1 ,2 ]
Gupta, P. K. [1 ]
机构
[1] Chaudhary Charan Singh Univ, Dept Genet & Plant Breeding, Meerut 250004, UP, India
[2] Chaudhary Charan Singh Univ, Dept Genet & Plant Breeding, Bioinformat Infrastruct Facil, Meerut 250004, Uttar Pradesh, India
[3] Univ Delhi South Campus, Dept Plant Mol Biol, New Delhi 110021, India
[4] Indian Inst Wheat & Barley Res IIWBR, Reg Stn, Shimla 171002, HP, India
[5] ICAR IARI, Div Genet & Plant Breeding, New Delhi 110012, India
关键词
Triticum aestivum; Leaf rust; Puccinia triticina; Lr28; Histone modifications; Gene expression; ChIP-seq; CIS-REGULATORY ELEMENTS; GENE-EXPRESSION; HISTONE H3; TRANSCRIPTION FACTOR; DNA METHYLATION; POLY(ADP-RIBOSE) POLYMERASE; ARABIDOPSIS-THALIANA; CPG METHYLATION; TIR DOMAINS; CELL-DEATH;
D O I
10.1007/s11103-020-01029-4
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Key Message Present study revealed a complex relationship among histone H3 methylation (examined using H3K4/K27me3 marks), cytosine DNA methylation and differential gene expression duringLr28mediated leaf rust resistance in wheat. During the present study, genome-wide histone modifications were examined in a pair of near isogenic lines (NILs) (with and withoutLr28in the background of cv. HD2329). The two histone marks used included H3K4me3 (an activation mark) and H3K27me3 (a repression mark). The results were compared with levels of expression (using RNA-seq) and DNA methylation (MeDIP) data obtained using the same pair of NILs. Some of the salient features of the present study include the following: (i) large scale differential binding sites (DBS) were available for only H3K4me3 in the susceptible cultivar, but for both H3K4me3 and H3K27me3 in its resistant NIL; (ii) DBSs for H3K27me3 mark were more abundant (> 80%) in intergenic regions, whereas DBSs for H3K4me3 were distributed in all genomic regions including exons, introns, intergenic, TTS (transcription termination sites) and promoters; (iii) fourteen (14) genes associated with DBSs showed co-localization for both the marks; (iv) only a small fraction (7% for H3K4me3 and 12% for H3K27me3) of genes associated with DBSs matched with the levels of gene expression inferred from RNA-seq data; (v) validation studies using qRT-PCR were conducted on 26 selected representative genes; results for only 11 genes could be validated. The proteins encoded by important genes involved in promoting infection included domains generally carried by R gene proteins such as Mlo like protein, protein kinases and purple acid phosphatase. Similarly, proteins encoded by genes involved in resistance included those carrying domains for lectin kinase, R gene, aspartyl protease, etc. Overall, the results suggest a very complex network of downstream genes that are expressed during compatible and incompatible interactions; some of the genes identified during the present study may be used in future validation studies involving RNAi/overexpression approaches.
引用
收藏
页码:113 / 136
页数:24
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