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针对集胞藻6803(Synechocystis sp. PCC 6803)的psbAII基因进行随机诱变,以鉴定光系统II反应中心D1蛋白中功能重要的残基。

Random mutagenesis targeted to the psbAII gene of Synechocystis sp. PCC 6803 to identify functionally important residues in the D1 protein of the photosystem II reaction center.

作者信息

Yamasato Akihiro, Kamada Tomoe, Satoh Kimiyuki

机构信息

Graduate School of Natural Science and Technology, Okayama University, Okayama, 700-8530 Japan.

出版信息

Plant Cell Physiol. 2002 May;43(5):540-8. doi: 10.1093/pcp/pcf066.

Abstract

More than one hundred mutants of Synechocystis sp. PCC 6803 impaired in photoautotrophic growth were generated by in vitro random PCR mutagenesis targeted to a region of the psbAII gene corresponding to a 210 amino acid (Ser148-Ala357) segment of the D1 protein. The 90 random mutants that could translate the full-length D1 protein carried 1-9 (on average 3.0) amino acid substitutions in the targeted region. Mutations were often found in the obligate photoheterotrophic strains at specific residues that have been reported or speculated to be important in the function of PSII, such as Y161, H198, H272, E333 and H337. This verifies the usefulness of the present method to identify functionally important residues in PSII. Other residues that were often mutated in the strains with impaired photoautotrophy included non-charged residues around the lumenal edges of transmembrane helices C, D and E, such as I192 and N296. Eleven mutants carried a single-point mutation in residues, such as Q165, Q187, W278, A294 and N298, and these identified the functional importance of these residues, most of which were on the donor side of PSII. A preliminary characterization of some of the mutants obtained in this study is provided.

摘要

通过针对psbAII基因中与D1蛋白210个氨基酸(Ser148 - Ala357)片段相对应的区域进行体外随机PCR诱变,产生了一百多个光合自养生长受损的集胞藻6803突变体。能够翻译全长D1蛋白的90个随机突变体在目标区域携带1 - 9个(平均3.0个)氨基酸替换。在专性光合异养菌株中,经常在已报道或推测对PSII功能重要的特定残基处发现突变,例如Y161、H198、H272、E333和H337。这验证了本方法在鉴定PSII中功能重要残基方面的有效性。在光合自养受损菌株中经常发生突变的其他残基包括跨膜螺旋C、D和E腔边缘周围的非带电残基,例如I192和N296。11个突变体在Q165、Q187、W278、A294和N298等残基处发生单点突变,这些突变确定了这些残基的功能重要性,其中大多数位于PSII的供体侧。本文提供了本研究中获得的一些突变体的初步表征。

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