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两个最近复制的玉米 NAC 转录因子同源物在响应炭疽菌侵染时被诱导表达。

Two recently duplicated maize NAC transcription factor paralogs are induced in response to Colletotrichum graminicola infection.

机构信息

Division of Biochemistry, Friedrich-Alexander-University Erlangen-Nuremberg, Staudtstrasse 5, D-91058 Erlangen, Germany.

出版信息

BMC Plant Biol. 2013 May 29;13:85. doi: 10.1186/1471-2229-13-85.

Abstract

BACKGROUND

NAC transcription factors belong to a large family of plant-specific transcription factors with more than 100 family members in monocot and dicot species. To date, the majority of the studied NAC proteins are involved in the response to abiotic stress, to biotic stress and in the regulation of developmental processes. Maize NAC transcription factors involved in the biotic stress response have not yet been identified.

RESULTS

We have found that two NAC transcription factors, ZmNAC41 and ZmNAC100, are transcriptionally induced both during the initial biotrophic as well as the ensuing necrotrophic colonization of maize leaves by the hemibiotrophic ascomycete fungus C. graminicola. ZmNAC41 transcripts were also induced upon infection with C. graminicola mutants that are defective in host penetration, while the induction of ZmNAC100 did not occur in such interactions. While ZmNAC41 transcripts accumulated specifically in response to jasmonate (JA), ZmNAC100 transcripts were also induced by the salicylic acid analog 2,6-dichloroisonicotinic acid (INA).To assess the phylogenetic relation of ZmNAC41 and ZmNAC100, we studied the family of maize NAC transcription factors based on the recently annotated B73 genome information. We identified 116 maize NAC transcription factor genes that clustered into 12 clades. ZmNAC41 and ZmNAC100 both belong to clade G and appear to have arisen by a recent gene duplication event. Including four other defence-related NAC transcription factors of maize and functionally characterized Arabidopsis and rice NAC transcription factors, we observed an enrichment of NAC transcription factors involved in host defense regulation in clade G. In silico analyses identified putative binding elements for the defence-induced ERF, Myc2, TGA and WRKY transcription factors in the promoters of four out of the six defence-related maize NAC transcription factors, while one of the analysed maize NAC did not contain any of these potential binding sites.

CONCLUSIONS

Our study provides a systematic in silico analysis of maize NAC transcription factors in which we propose a nomenclature for maize genes encoding NAC transcription factors, based on their chromosomal position. We have further identified five pathogen-responsive maize NAC transcription factors that harbour putative binding elements for other defence-associated transcription factors in the proximal promoter region, indicating an involvement of the described NACs in the maize defence network. Our phylogenetic analysis has revealed that the majority of the yet described pathogen responsive NAC proteins from all plant species belong to clade G and suggests that they are phylogenetically related.

摘要

背景

NAC 转录因子属于植物特有的转录因子大家族,在单子叶和双子叶物种中超过 100 个家族成员。迄今为止,大多数研究的 NAC 蛋白都参与了非生物胁迫、生物胁迫和发育过程的调节。参与生物胁迫反应的玉米 NAC 转录因子尚未被鉴定。

结果

我们发现,两个 NAC 转录因子,ZmNAC41 和 ZmNAC100,在半生物性真菌 C. graminicola 最初的生物亲和以及随后的坏死亲和定殖过程中,转录水平都被诱导。ZmNAC41 的转录本也在感染宿主穿透缺陷的 C. graminicola 突变体时被诱导,而 ZmNAC100 的诱导则不会发生在这种相互作用中。虽然 ZmNAC41 的转录本特异性地响应茉莉酸(JA)积累,但 ZmNAC100 的转录本也被水杨酸类似物 2,6-二氯异烟酸(INA)诱导。为了评估 ZmNAC41 和 ZmNAC100 的系统发育关系,我们基于最近注释的 B73 基因组信息研究了玉米 NAC 转录因子家族。我们鉴定了 116 个玉米 NAC 转录因子基因,它们聚类为 12 个分支。ZmNAC41 和 ZmNAC100 都属于分支 G,似乎是由最近的基因复制事件产生的。包括玉米的其他四个防御相关的 NAC 转录因子和功能表征的拟南芥和水稻 NAC 转录因子,我们观察到在分支 G 中富集了参与宿主防御调节的 NAC 转录因子。计算机分析在四个防御相关的玉米 NAC 转录因子的启动子中鉴定了防御诱导的 ERF、Myc2、TGA 和 WRKY 转录因子的可能结合元件,而分析的玉米 NAC 中的一个则没有这些潜在的结合位点。

结论

我们的研究提供了一个系统的玉米 NAC 转录因子的计算分析,在此基础上,我们根据它们在染色体上的位置,提出了一个玉米编码 NAC 转录因子的命名方案。我们进一步鉴定了五个对病原体有反应的玉米 NAC 转录因子,它们在近端启动子区域有其他防御相关转录因子的潜在结合元件,表明所描述的 NAC 参与了玉米防御网络。我们的系统发育分析表明,来自所有植物物种的大多数已描述的对病原体有反应的 NAC 蛋白都属于分支 G,并表明它们在系统发育上是相关的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/73fb/3694029/5e10776a823b/1471-2229-13-85-1.jpg

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