Combination of Trp and Glu residues for recognition of mRNA cap structure Analysis of m7G base recognition site of human cap binding protein (IF‐4E) by site‐directed mutagenesis

Doi Mitsunobu; Inoue Masatoshi; Ishida Toshimasa; Iyo Hiromi; Morioka Hiroshi; Nishikawa Satoshi; Tanaka Toshiki; Ueda Hitoshi; Uesugi Seiichi

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Combination of Trp and Glu residues for recognition of mRNA cap structure Analysis of m7G base recognition site of human cap binding protein (IF‐4E) by site‐directed mutagenesis

机译：Trp和Glu残基的结合用于识别mRNA帽结构通过定点诱变分析人帽结合蛋白（IF-4E）的m7G碱基识别位点

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>Four mutants of the human cap binding protein (hCBP), in which Trp-102, Glu-103, Asp-104 or Glu-105 was changed to the aliphatic Leu or Ala, were prepared, and their cap binding abilities were examined. Cap binding abilities of two mutants. W102L (Trp-102→Leu) and E105A (Glu-105→Ala), were significantly decreased in comparison with the wild-type hCBP. This result suggest that Trp-102 and Glu-105 are both necessary for the cap binding, and the most probable binding mode with the m7G of cap structure is the combination of the stacking by Trp-102 and the hydrogen-bond pairing by Glu-105, as was already proposed from the model studies.

机译：>制备了四个人类帽结合蛋白（hCBP）突变体，其中Trp-102，Glu-103，Asp-104或Glu-105变为脂肪族亮氨酸或丙氨酸，它们的帽结合能力为检查。两个突变体的帽结合能力。与野生型hCBP相比，W102L（Trp-102→Leu）和E105A（Glu-105→Ala）显着降低。这个结果表明，Trp-102和Glu-105都是帽结合所必需的，并且帽结构的m 7 G的最可能结合方式是Trp-102的堆叠和通过模型研究已经提出的通过Glu-105进行的氢键配对。

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《FEBS Letters》 |1991年第2期|共页
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Doi Mitsunobu; Inoue Masatoshi; Ishida Toshimasa; Iyo Hiromi; Morioka Hiroshi; Nishikawa Satoshi; Tanaka Toshiki; Ueda Hitoshi; Uesugi Seiichi;
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中图分类分子生物学;
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7. Combination of Trp and Glu residues for recognition of mRNA cap structure Analysis of m7G base recognition site of human cap binding protein (IF-4E) by site-directed mutagenesis [O] . Ueda Hitoshi, Iyo Hiromi, Doi Mitsunobu, 1991

机译：Trp和Glu残基的结合用于mRNA帽结构的识别通过定点诱变分析人帽结合蛋白（IF-4E）的m7G碱基识别位点

Combination of Trp and Glu residues for recognition of mRNA cap structure Analysis of m7G base recognition site of human cap binding protein (IF‐4E) by site‐directed mutagenesis

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