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小麦(普通小麦)的液泡半胱氨酸蛋白酶在不同因素诱导的叶片衰老中普遍存在。

Vacuolar cysteine proteases of wheat (Triticum aestivum L.) are common to leaf senescence induced by different factors.

作者信息

Martínez Dana E, Bartoli Carlos G, Grbic Vojislava, Guiamet Juan J

机构信息

Instituto de Fisiología Vegetal, Universidad Nacional de La Plata, cc 327, 1900-La Plata, Argentina.

出版信息

J Exp Bot. 2007;58(5):1099-107. doi: 10.1093/jxb/erl270. Epub 2007 Jan 11.

DOI:10.1093/jxb/erl270
PMID:17218544
Abstract

Cellular proteins are extensively degraded during leaf senescence, and this correlates with an up-regulation of protease gene expression, particularly cysteine proteases. The objectives of this work were (i) to detect cysteine proteases associated with senescence of wheat leaves under different conditions and (ii) to find out their subcellular location. Activity labelling of cysteine proteases with the biotinylated inhibitor DCG-04 detected five bands at 27, 36, 39, 42, and 46 kDa in leaves of wheat senescing under continuous darkness. In-gel activity assays showed that these proteases are only active in an acid milieu (pH 4), and their activity increased several-fold in senescing leaves. Fractionation experiments showed that the senescence-associated cysteine proteases of 36, 39, 42, and 46 kDa localize to a vacuolar-enriched fraction. The vacuolar cysteine proteases of 36, 39, and 42 kDa increased in activity in attached flag leaves senescing naturally during post-anthesis, and in attached leaves of plants subjected to a period of water deficit. Thus, the activity of these vacuolar cysteine proteases is associated with developmental (post-anthesis) senescence and with senescence induced by stress factors (i.e. protracted darkness or drought). This suggests that vacuoles are involved in senescence-associated cellular degradation, and that different senescence-inducing factors may converge on a single degradation pathway.

摘要

在叶片衰老过程中,细胞蛋白质会被大量降解,这与蛋白酶基因表达上调相关,尤其是半胱氨酸蛋白酶。本研究的目的是:(i)检测不同条件下与小麦叶片衰老相关的半胱氨酸蛋白酶;(ii)确定其亚细胞定位。用生物素化抑制剂DCG-04对半胱氨酸蛋白酶进行活性标记,在持续黑暗条件下衰老的小麦叶片中检测到27、36、39、42和46 kDa的五条带。凝胶内活性分析表明,这些蛋白酶仅在酸性环境(pH 4)中有活性,且其活性在衰老叶片中增加了数倍。分级分离实验表明,36、39、42和46 kDa与衰老相关的半胱氨酸蛋白酶定位于富含液泡的组分中。在花后自然衰老的旗叶以及经历一段时间水分亏缺的植株的附着叶片中,36、39和42 kDa的液泡半胱氨酸蛋白酶活性增加。因此,这些液泡半胱氨酸蛋白酶的活性与发育(花后)衰老以及由胁迫因素(即长时间黑暗或干旱)诱导的衰老相关。这表明液泡参与了与衰老相关的细胞降解,并且不同的衰老诱导因素可能汇聚到单一的降解途径上。

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