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莱茵衣藻的CPH1基因编码两种隐花色素,其水平受光诱导的蛋白水解作用控制。

The CPH1 gene of Chlamydomonas reinhardtii encodes two forms of cryptochrome whose levels are controlled by light-induced proteolysis.

作者信息

Reisdorph Nichole A, Small Gary D

机构信息

Cellular and Molecular Biology Group, University of South Dakota, Vermillion, South Dakota 57069, USA.

出版信息

Plant Physiol. 2004 Apr;134(4):1546-54. doi: 10.1104/pp.103.031930. Epub 2004 Apr 2.

Abstract

Cryptochromes are proteins related to DNA photolyases and have been shown to function as blue-light photoreceptors and to play important roles in circadian rhythms in both plants and animals. The CPH1 gene from Chlamydomonas reinhardtii was originally predicted to encode a putative cryptochrome protein of 867 amino acids with a predicted molecular mass of 91 kD (Small et al., 1995). However, western blotting with antibodies specific to the CPH1 protein revealed the presence of two proteins that migrate at apparent molecular mass of approximately 126 and 143 kD. A reexamination of the assigned intron-exon boundaries has shown that the previously assigned intron 7 is in fact part of exon 7 which leads to a predicted protein of 1,007 amino acids corresponding to a size of 104.6 kD. The two forms of CPH1 that migrate slower on SDS-PAGE presumably result from unknown posttranslational modifications. In C. reinhardtii cells synchronized by light to dark cycles, the two slow migrating forms of CPH1 protein accumulate in the dark and disappear rapidly in the light. Both red and blue light are effective at inducing the degradation of the CPH1 proteins. Proteasomes are implicated because degradation is inhibited by MG132, a proteasome inhibitor. Studies with deletion mutants indicate that the C-terminal region is important for both the posttranslational modification and the protein's stability under both light and dark conditions.

摘要

隐花色素是与DNA光解酶相关的蛋白质,已被证明可作为蓝光光感受器,并在植物和动物的昼夜节律中发挥重要作用。莱茵衣藻的CPH1基因最初被预测编码一种推定的隐花色素蛋白,含有867个氨基酸,预测分子量为91kD(Small等人,1995年)。然而,用针对CPH1蛋白的特异性抗体进行蛋白质印迹分析显示存在两种蛋白质,其表观分子量约为126kD和143kD。对指定的内含子-外显子边界进行重新检查表明,先前指定的内含子7实际上是外显子7的一部分,这导致预测的蛋白质含有1,007个氨基酸,对应大小为104.6kD。在SDS-PAGE上迁移较慢的两种CPH1形式可能是由未知的翻译后修饰导致的。在通过明暗循环同步的莱茵衣藻细胞中,两种迁移较慢的CPH1蛋白形式在黑暗中积累,并在光照下迅速消失。红光和蓝光都能有效诱导CPH1蛋白的降解。蛋白酶体与之相关,因为降解被蛋白酶体抑制剂MG132抑制。对缺失突变体的研究表明,C末端区域对于翻译后修饰以及蛋白质在光照和黑暗条件下的稳定性都很重要。

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