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ACT结构域重复蛋白7(ACR7)在水稻细胞核中与伴侣蛋白HSP18.0-CII相互作用。

ACT domain repeat protein 7, ACR7, interacts with a chaperone HSP18.0-CII in rice nuclei.

作者信息

Hayakawa Toshihiko, Kudo Toru, Ito Takashi, Takahashi Nobuyuki, Yamaya Tomoyuki

机构信息

Graduate School of Agricultural Science, Tohoku University, 1-1 Tsutsumidori-Amamiyamachi, Aoba-ku, Sendai, 981-8555 Japan.

出版信息

Plant Cell Physiol. 2006 Jul;47(7):891-904. doi: 10.1093/pcp/pcj062. Epub 2006 May 23.

DOI:10.1093/pcp/pcj062
PMID:16720649
Abstract

The regulatory ACT domains serve as amino acid-binding sites in some amino acid metabolic enzymes and transcriptional regulators in bacteria. To elucidate the molecular roles of the glutamine (Gln)-sensing system in nitrogen (N) metabolism in plants, we isolated six genes encoding ACT domain repeat proteins (ACR1, and ACR5-ACR9) from rice (Oryza sativa L.) using genomic information on the primary structure composed of four copies of the domain homologous to those of bacterial Gln sensor GLND. Since expression of ACR7 was the most abundant of the six ACR orthologous genes, we focused on this ACR in the current study. Gene products of ACR7 were most abundant in young developing leaf blades of rice, and ACR7 protein is specifically localized in the nucleus of the parenchyma cells of phloem and xylem in the vascular bundles. A yeast two-hybrid screen identified a small heat stress protein (HSP18.0-CII) as a protein interacting with ACR7. Transient expression analysis of HSP18.0-CII:sGFP in cultured rice cells, followed by co-immunoprecipitation, suggests that the nuclear ACR7 indeed interacted with nucleocytoplasmic HSP18.0-CII in vivo. The potential ability of nuclear protein ACR7 to bind Gln and the possibility of the protein acting as a Gln sensor in rice leaves is discussed.

摘要

调控性ACT结构域在细菌的一些氨基酸代谢酶和转录调节因子中作为氨基酸结合位点。为了阐明植物氮(N)代谢中谷氨酰胺(Gln)感知系统的分子作用,我们利用与细菌Gln传感器GLND结构域同源的由四个拷贝组成的一级结构的基因组信息,从水稻(Oryza sativa L.)中分离出六个编码ACT结构域重复蛋白的基因(ACR1以及ACR5 - ACR9)。由于ACR7的表达在六个ACR同源基因中最为丰富,我们在当前研究中聚焦于该ACR。ACR7的基因产物在水稻幼嫩的发育叶片中最为丰富,并且ACR7蛋白特异性定位于维管束中韧皮部和木质部薄壁细胞的细胞核中。酵母双杂交筛选鉴定出一种小热激蛋白(HSP18.0 - CII)作为与ACR7相互作用的蛋白。在培养的水稻细胞中对HSP18.0 - CII:sGFP进行瞬时表达分析,随后进行免疫共沉淀,结果表明细胞核中的ACR7在体内确实与核质中的HSP18.0 - CII相互作用。本文讨论了核蛋白ACR7结合Gln的潜在能力以及该蛋白在水稻叶片中作为Gln传感器发挥作用的可能性。

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