首页> 美国卫生研究院文献>Journal of Bacteriology >A Second and Unusual pucBA Operon of Rhodobacter sphaeroides 2.4.1: Genetics and Function of the Encoded Polypeptides
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A Second and Unusual pucBA Operon of Rhodobacter sphaeroides 2.4.1: Genetics and Function of the Encoded Polypeptides

机译:球形红球菌第二个和异常的pucBA操纵子2.4.1:编码多肽的遗传和功能

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摘要

A new operon (designated the puc2BA operon) displaying a high degree of similarity to the original pucBA genes of Rhodobacter sphaeroides 2.4.1 (designated puc1) was identified and studied genetically and biochemically. The puc2B-encoded polypeptide is predicted to exhibit 94% identity with the original β-apoprotein. The puc2A-encoded polypeptide is predicted to be much larger (263 amino acids) than the 54-amino-acid puc1A-encoded polypeptide. In the first 48 amino acids of the puc2A-encoded polypeptide there is 58% amino acid sequence identity to the original puc1A-encoded polypeptide. We found that puc2BA is expressed, and DNA sequence data suggested that puc2BA is regulated by the PpsR/AppA repressor-antirepressor and FnrL. Employing genetic and biochemical approaches, we obtained evidence that the puc2B-encoded polypeptide is able to enter into LH2 complex formation, but neither the full-length puc2A-encoded polypeptide nor its N-terminal 48-amino-acid derivative is able to enter into LH2 complex formation. Thus, the sole source of α-polypeptides for the LH2 complex is puc1A. The role of the puc1C-encoded polypeptide was also determined. We found that the presence of this polypeptide is essential for normal levels of transcription and translation of the puc1 operon but not for transcription and translation of the puc2 operon. Thus, the puc1C gene product appears to have both transcriptional and posttranscriptional roles in LH2 formation. Finally, the absence of any LH2 complex when puc1B was deleted in frame was surprising since we know that in the presence of functional puc2BA, approximately 30% of the LH2 complexes normally observed contain a puc2B-encoded β-polypeptide.
机译:鉴定了一种新的操纵子(称为puc2BA操纵子),该操纵子与球形红球菌2.4.1的原始pucBA基因(称为puc1)具有高度相似性,并进行了遗传和生化研究。预测puc2B编码的多肽与原始β-载脂蛋白具有94%的同一性。预测puc2A编码的多肽(263个氨基酸)比54个氨基酸的puc1A编码的多肽大得多。在puc2A编码的多肽的前48个氨基酸中,与原始puc1A编码的多肽有58%的氨基酸序列同一性。我们发现puc2BA表达,并且DNA序列数据表明puc2BA受PpsR / AppA阻遏物-抗阻遏物和FnrL调控。利用遗传和生化方法,我们获得了puc2B编码的多肽能够进入LH2复合体形成的证据,但是全长puc2A编码的多肽或其N端48个氨基酸衍生物都无法进入LH2复合物的形成。因此,用于LH2复合物的唯一α多肽来源是puc1A。还确定了puc1C编码多肽的作用。我们发现,该多肽的存在对于puc1操纵子的正常转录和翻译水平至关重要,而对于 puc2 操纵子的转录和翻译则不是必需的。因此, puc1C 基因产物似乎在LH2的形成中具有转录和转录后作用。最后,当在框架中删除 puc1B 时不存在任何LH2复合体是令人惊讶的,因为我们知道在存在功能性 puc2BA 的情况下,通常观察到大约30%的LH2复合体包含一个 puc2B 编码的β-多肽。

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