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通过基因改造提高萤火虫荧光素酶的生物发光强度。

Increase in bioluminescence intensity of firefly luciferase using genetic modification.

作者信息

Fujii Hiroya, Noda Kenichi, Asami Yasuo, Kuroda Akio, Sakata Minoru, Tokida Akihiko

机构信息

Bussan Nanotech Research Institute Inc., Tsukuba, Ibaraki 305-0074, Japan.

出版信息

Anal Biochem. 2007 Jul 15;366(2):131-6. doi: 10.1016/j.ab.2007.04.018. Epub 2007 Apr 18.

Abstract

Firefly luciferase is widely used for enzymatic measurement of ATP, and its gene is used as a reporter for gene expression experiments. From our mutant library, we selected novel mutations in Photinus pyralis luciferase with higher luminescence intensity. These included mutations at Ile423, Asp436, and Leu530. Luciferase is structurally composed of a large N-terminal active site domain (residues 1-436), a flexible linker (residues 436-440) peptide, and a small C-terminal domain (residues 440-550) facing the N domain. Thus, the mutations are located at the junction of the N-terminal domain and the flexible linker, in the flexible linker peptide, and in the tip of the C-terminal domain, respectively. Substitution of Asp436 with a nonbulky amino acid such as Gly remarkably increased the substrate affinity for ATP and d-luciferin. Substitution of Ile423 with a hydrophobic amino acid such as Leu and that of Leu530 with a positively charged amino acid such as Arg increased the substrate affinity and the turnover rate. Combining these mutations, we obtained luciferases that generate more than 10-fold higher luminescence intensity than the wild-type enzyme.

摘要

萤火虫荧光素酶被广泛用于ATP的酶促检测,其基因被用作基因表达实验的报告基因。我们从突变体文库中筛选出了发光强度更高的新的北美萤火虫荧光素酶突变体。这些突变包括位于Ile423、Asp436和Leu530位点的突变。荧光素酶在结构上由一个大的N端活性位点结构域(第1至436位氨基酸残基)、一个柔性连接肽(第436至440位氨基酸残基)和一个面向N结构域的小的C端结构域(第440至550位氨基酸残基)组成。因此,这些突变分别位于N端结构域与柔性连接肽的交界处、柔性连接肽内以及C端结构域的末端。用诸如甘氨酸这样的非庞大氨基酸取代Asp436显著提高了对ATP和d-荧光素的底物亲和力。用诸如亮氨酸这样的疏水氨基酸取代Ile423以及用诸如精氨酸这样的带正电荷氨基酸取代Leu530提高了底物亲和力和周转速率。将这些突变组合起来,我们获得了发光强度比野生型酶高出10倍以上的荧光素酶。

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