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非洲爪蟾TFIIIA对体细胞5S rRNA基因转录的特异性受限。

Restricted specificity of Xenopus TFIIIA for transcription of somatic 5S rRNA genes.

作者信息

Ghose Romi, Malik Mariam, Huber Paul W

机构信息

Department of Chemistry and Biochemistry, University of Notre Dame, Notre Dame, Indiana 46556, USA.

出版信息

Mol Cell Biol. 2004 Mar;24(6):2467-77. doi: 10.1128/MCB.24.6.2467-2477.2004.

DOI:10.1128/MCB.24.6.2467-2477.2004
PMID:14993284
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC355861/
Abstract

Xenopus transcription factor IIIA (TFIIIA) is phosphorylated on serine-16 by CK2. Replacements with alanine or glutamic acid were made at this position in order to address the question of whether phosphorylation possibly influences the function of this factor. Neither substitution has an effect on the DNA or RNA binding activity of TFIIIA. The wild-type factor and the alanine variant activate transcription of somatic- and oocyte-type 5S rRNA genes in nuclear extract immunodepleted of endogenous TFIIIA. The glutamic acid variant (S16E) supports the transcription of somatic-type genes at levels comparable to those of wild-type TFIIIA; however, there is no transcription of the oocyte-type genes. This differential behavior of the phosphomimetic mutant protein is also observed in vivo when using early-stage embryos, where this mutant failed to activate transcription of the endogenous oocyte-type genes. Template exclusion assays establish that the S16E mutant binds to the oocyte-type 5S rRNA genes and recruits at least one other polymerase III transcription factor into an inactive complex. Phosphorylation of TFIIIA by CK2 may allow the factor to continue to act as a positive activator of the somatic-type genes and simultaneously as a repressor of the oocyte-type 5S rRNA genes, indicating that there is a mechanism that actively promotes repression of the oocyte-type genes at the end of oogenesis.

摘要

非洲爪蟾转录因子IIIA(TFIIIA)在丝氨酸16位点被酪蛋白激酶2(CK2)磷酸化。为了研究磷酸化是否可能影响该因子的功能,在此位置用丙氨酸或谷氨酸进行了替换。两种替换对TFIIIA的DNA或RNA结合活性均无影响。野生型因子和丙氨酸变体在去除内源性TFIIIA的核提取物中可激活体细胞型和卵母细胞型5S rRNA基因的转录。谷氨酸变体(S16E)支持体细胞型基因的转录,其水平与野生型TFIIIA相当;然而,卵母细胞型基因不发生转录。当使用早期胚胎时,在体内也观察到了这种拟磷酸化突变蛋白的不同行为,该突变体未能激活内源性卵母细胞型基因的转录。模板排除试验表明,S16E突变体与卵母细胞型5S rRNA基因结合,并将至少一种其他聚合酶III转录因子募集到一个无活性的复合物中。CK2对TFIIIA的磷酸化可能使该因子继续作为体细胞型基因的正激活因子,同时作为卵母细胞型5S rRNA基因的阻遏物,这表明存在一种机制,在卵子发生末期积极促进对卵母细胞型基因的抑制。

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The mitogen-activated protein (MAP) kinase ERK induces tRNA synthesis by phosphorylating TFIIIB.有丝分裂原激活蛋白(MAP)激酶ERK通过磷酸化TFIIIB诱导tRNA合成。
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