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编码水母发光蛋白同种型的互补DNA的序列比较。

Sequence comparisons of complementary DNAs encoding aequorin isotypes.

作者信息

Prasher D C, McCann R O, Longiaru M, Cormier M J

出版信息

Biochemistry. 1987 Mar 10;26(5):1326-32. doi: 10.1021/bi00379a019.

DOI:10.1021/bi00379a019
PMID:2882777
Abstract

Aequorin is the Ca2+-activated photoprotein which participates in the bioluminescence from the circumoral ring of the hydromedusa Aequorea victoria. The nucleotide sequences of five aequorin cDNAs have been compared and shown to code for three aequorin isoforms. The cDNA AEQ1 contains the entire protein coding region of 196 amino acids. The other four cDNAs contain only 70-90% of the coding region and apparently code for at least two other isoforms whose amino acid sequences differ significantly from that encoded by AEQ1. The nucleotide sequences coding for the three isotypes differ at a minimum of 54 positions out of a total of 588 nucleotides necessary to code for apoaequorin. Of these nucleotide differences, 24 account for 23 amino acid replacements, substantiating the microheterogeneity observed during sequencing of purified native aequorin [Charbonneau, H., Walsh, K.A., McCann, R.O., Prendergast, F.G., Cormier, M.J., & Vanaman, T.C. (1985) Biochemistry 24, 6762-6771]. Comparison of the deduced cDNA translations with the native protein sequences suggests the loss of seven residues from the amino terminus during purification of aequorin from Aequorea. Aequorin rapidly extracted from the jellyfish using conditions to minimize proteolysis is shown to have a larger molecular weight than that of purified native aequorin. Escherichia coli expressed aequorin encoded by AEQ1 is shown to have the same molecular weight and isoelectric point as those of one of the isotypes rapidly extracted from Aequorea.

摘要

水母发光蛋白是一种Ca2+激活的光蛋白,参与了维多利亚多管水母口周环的生物发光过程。已对五个水母发光蛋白cDNA的核苷酸序列进行了比较,结果表明它们编码三种水母发光蛋白同工型。cDNA AEQ1包含196个氨基酸的完整蛋白质编码区。其他四个cDNA仅包含70 - 90%的编码区,显然编码至少另外两种同工型,其氨基酸序列与AEQ1编码的序列有显著差异。编码这三种同工型的核苷酸序列在编码脱辅基水母发光蛋白所需的总共588个核苷酸中至少有54个位置不同。在这些核苷酸差异中,24个差异导致了23个氨基酸替换,证实了在纯化天然水母发光蛋白测序过程中观察到的微异质性[Charbonneau, H., Walsh, K.A., McCann, R.O., Prendergast, F.G., Cormier, M.J., & Vanaman, T.C. (1985) Biochemistry 24, 6762 - 6771]。将推导的cDNA翻译序列与天然蛋白质序列进行比较表明,从维多利亚多管水母中纯化水母发光蛋白的过程中,其氨基末端有七个残基丢失。在尽量减少蛋白水解的条件下从水母中快速提取的水母发光蛋白,其分子量比纯化的天然水母发光蛋白大。由AEQ1编码的大肠杆菌表达的水母发光蛋白,其分子量和等电点与从维多利亚多管水母中快速提取的一种同工型相同。

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1
Sequence comparisons of complementary DNAs encoding aequorin isotypes.编码水母发光蛋白同种型的互补DNA的序列比较。
Biochemistry. 1987 Mar 10;26(5):1326-32. doi: 10.1021/bi00379a019.
2
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Cloning and expression of the cDNA coding for aequorin, a bioluminescent calcium-binding protein.编码水母发光蛋白(一种生物发光钙结合蛋白)的cDNA的克隆与表达。
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Use of recombinant biotinylated aequorin in microtiter and membrane-based assays: purification of recombinant apoaequorin from Escherichia coli.重组生物素化水母发光蛋白在微量滴定和基于膜的分析中的应用:从大肠杆菌中纯化重组脱辅基水母发光蛋白。
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Bioluminescent immunoassay using a fusion protein of protein A and the photoprotein aequorin.使用蛋白A与光蛋白水母发光蛋白的融合蛋白进行生物发光免疫测定。
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Bioluminescent and biochemical properties of Cys-free Ca-regulated photoproteins obelin and aequorin.无半胱氨酸钙调节的生物发光和生物化学特性的光蛋白 obelin 和 aequorin。
J Photochem Photobiol B. 2017 Sep;174:97-105. doi: 10.1016/j.jphotobiol.2017.07.021. Epub 2017 Jul 23.

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