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二种多管水母光蛋白基因的分离、表达及生物活性初步研究

, PP. 110-117

Keywords: 大型多管水母,细小多管水母,光蛋白基因,表达

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Abstract:

分别从厦门东海域的大型多管水母和细小多管水母中分离到了新的光蛋白基因aeqxm和aeqxxm,并在大肠杆菌中进行了表达.aeqxm和aeqxxmDNA序列的编码区总长均为585bp,无内含子序列,推导的氨基酸序列总长均为195个氨基酸.aeqxm,aeqxxmDNA和AEVAQ440XcDNA之间的核苷酸序列同源性分别为80.7%,85.1%,aeqxm和aeqxxmDNA的核苷酸序列同源性为87.2%.原光蛋白apoaeqxm,apoaeqxxm与AEVAQ440X编码的氨基酸序列之间的同源性分别为84.7%,84.2%,apoaeqxm和apoaeqxxm的氨基酸序列之间的同源性为94.4%.分别将aeqxm和aeqxxm基因克隆至pTO-T7表达载体,apoaeqxm,apoaeqxxm在大肠杆菌中的表达量都达到40%左右.取菌体超声上清与腔肠动物荧光素f、巯基乙醇混合再生后,加入CaCl2,用荧光全谱仪检测到470nm处的瞬时发光,表明表达的apoaeqxm,apoaeqxxm具有正常的生物学功能.

 References

[1]  SALA-NEWBY G B, TAYLOR K M, BADMINTON M N, et al. Imaging bioluminescent indicators show Ca2+ and ATP permeability thresholds in live cells attacked by complement [J]. Immunology, 1998, 93: 601-609.
[2]  HAMPTON T G, AMENDE I, TRAVERS K E, et al. Intracellular calcium dynamics in mouse model of myocardial stunning [J]. Am J Physiol, 1998, 274: H1821-7.
[3]  CESSNA S G, CHANDRA S, LOW P S. Hypo-osmotic shock of tobacco cells stimulates Ca2 + fluxes deriving first from external and then internal Ca2+ stores [J]. J Biol Chem, 1998, 273:27 286- 27 291.
[4]  CASADEI J, POWELL M J, KENTEN J H. Expression and secretion of aequorin as a chimeric antibody by means of a mammalian expression vector [J]. Proc Natl Acad Sci USA, 1990, 87:2 047-2 051.
[5]  VERHAEGEN M, CHRISTOPOULOS T K. Quantitative polymerase chain reaction based on a dual-analyte chemiluminescence hybridization assay for target DNA and internal standard [J]. Anal Chem, 1998, 70:4 120-4 125.
[6]  INOUYE S, NOGUCHI M, SAKAKI Y, et al. Cloning and sequence analysis of cDNA for the luminescent protein aequorin[J]. Proc Natl Acad Sci USA, 1985, 82:3 154-3 158.
[7]  CHARBONNEAU H, WALSH K A, MCCANN R O, et al. Amino acid sequence of the calcium-dependent photoprotein aequorin [J]. American Chemical Society, 1985, 24:6 762-6 771.
[8]  萨姆布鲁克J,弗里奇E F,曼尼阿蒂斯T.分子克隆操作指南(第二版)[M].金冬雁,黎孟枫等译.北京:科学出版社,1992.
[9]  SHIMOMURA O, JOHNSON F H. Regeneration of the photoprotein aequorin [J]. Nature, 1975, 17; 256(5514):236-238.
[10]  NOMURA M, INOUYE S, OHMIYA Y, et al. A C-terminal proline is required for bioluminescence of the Ca2+-binding photoprotein, aequorin [J]. FEBS Lett, 1991, 295: 63-66.
[11]  KUROSE K, INOUYE S, SAKAKI Y, et al. Bioluminescence of the Ca2+-binding photoprotein aequorin after cysteine modification [J]. Proc Natl Acad Sci USA, 1989, 86: 80-84.
[12]  LEUNG C F, WEBB S E, MILLER A L. Calcium transients accompany ooplasmic segregation in zebrafish embryos [ J ].Dev Growth Differ, 1998, 40: 313-326.
[13]  ZENNO S, INOUYE S. Bioluminescent immunoassay using a fusion protein of protein A and the photoprotein aequorin [J].Biochem Biophys Res Commun, 1990, 171: 169-174.
[14]  ACTOR J K, KUFFNER T, DEZZUTTI C S, et al. A flash-type bioluminescent immunoasasy that is more sensitive than radioimaging: quantitative detection of cytokine cDNA in activated and resting human cells [J]. J Immunol Methods, 1998,211: 65-77.
[15]  INOUYE S, SAKAKI Y, GOTO T, et al. Expression of apoaequorin complementary DNA in Escherichia coli [J]. Biochemistry, 1986, 25:8 425-8 429.
[16]  PRASHER D, MCCANN R O, CORMIER M J. Cloning and expression of the cDNA cloning for aequorin: a bioluminescent calcium-binding protein [J]. Biochem Biophys Res Commun, 1985, 126(3): 1 295-1 268.
[17]  罗文新,张军,夏宁邵,等.一种带增强子的原核高效表达载体的构建及初步应用[J].生物工程学报,2000,16(5):578-581.
[18]  CORMIER M J, PRASHER D C, LONGIARU M, et al. The erzymology and molecular biology of the Ca2 + activated photoprotein, aequorin [J]. Photochem Photobiol, 1989, 49: 59-512.
[19]  SHIMOMURA O, INOUYE S, MUSICKI B, et al. Recombinant aequorin and recombinant semi-synthetic aequorins: cellular Ca2+ ion indicators [J]. Biochem J, 1990, 270: 309-312.

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