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首页> 外文期刊>Plant Science: An International Journal of Experimental Plant Biology >Cloning of a cystatin gene from sugar beet M14 that can enhance plant salt tolerance
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Cloning of a cystatin gene from sugar beet M14 that can enhance plant salt tolerance

机译:从甜菜M14克隆可提高植物耐盐性的胱抑素基因

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摘要

An open reading frame encoding a cysteine protease inhibitor, cystatin was isolated from the buds of sugar beet monosomic addition line M14 (ByM14) using 5'-/3'-RACE method. It encoded a polypeptide of 104 amino acids with conserved G and PW motifs, the consensus phytocystatin sequence LARFAV and the active site QVVAG. The protein showed significant homology to other plant cystatins. BvM14-cystatin was expressed ubiquitously in roots, stems, leaves and flower tissues with relatively high abundance in developing stems and roots. It was found to be localized in the nucleus, cytoplasm and plasma membrane. Recombinant BvM14-cystatin expressed in Escherichia coli was purified and it exhibited cysteine protease inhibitor activity. Salt-stress treatment induced BvM14-cystatin transcript levels in the M14 seedlings. Homozygous Arabidopsis plants over-expressing ByM14-cystatin showed enhanced salt tolerance. Taken together, these data improved understanding of the functions of BvM14-cystatin and highlighted the possibility of employing the cystatin in engineering plants for enhanced salt tolerance.
机译:使用5'-/ 3'-RACE方法从甜菜单体附加系M14(ByM14)的芽中分离出编码半胱氨酸蛋白酶抑制剂胱抑素的开放阅读框。它编码了一个具有104个氨基酸的多肽,具有保守的G和PW基序,植物胱抑素共有序列LARFAV和活性位点QVVAG。该蛋白显示出与其他植物半胱氨酸蛋白酶的显着同源性。 BvM14-胱抑素普遍存在于根,茎,叶和花组织中,在发育中的茎和根中相对较高。发现它位于细胞核,细胞质和质膜中。纯化了在大肠杆菌中表达的重组BvM14-胱抑素,并显示出半胱氨酸蛋白酶抑制剂的活性。盐胁迫诱导了M14幼苗中BvM14-胱抑素的转录水平。过表达ByM14-胱抑素的纯合拟南芥植物显示增强的耐盐性。综上所述,这些数据增进了对BvM14-胱抑素功能的理解,并突出了在工程植物中使用胱抑素以增强盐耐受性的可能性。

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