A STUDY OF SENSITIZED LANTHANIDE LUMINESCENCE IN AN ENGINEERED CALCIUM-BINDING PROTEIN

被引:16
作者
CLARK, ID
MACMANUS, JP
BANVILLE, D
SZABO, AG
机构
[1] NATL RES COUNCIL CANADA, INST BIOL SCI, MONTREAL RD, OTTAWA K1A 0R6, ONTARIO, CANADA
[2] NATL RES COUNCIL CANADA, BIOTECHNOL RES INST, MONTREAL H4P 2R2, PQ, CANADA
关键词
D O I
10.1006/abio.1993.1142
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
In this study, the CD loop of the Ca2+-binding protein oncomodulin was replaced by a high-affinity, metal-binding sequence that was found to reverse the order of fill of the two sites in the protein. A cysteine was included at position 7 of this sequence, i.e., DKNADGCIEFEE. The cysteine allowed covalent attachment of chromophores to the loop that could subsequently be tested for their ability to sensitize the luminescence of Tb3+ or Eu3+ bound in the loop. 7-Diethylamino-3-((4'iodoacetylamino)phenyl)-4-methylcoumarin was the most efficient Eu3+ sensitizer studied, consistent with a mechanism of energy transfer that involves the triplet state of the donor. 4-Iodoacetamidosalicylic acid was the most efficient Tb3+ donor tested. Levels of lanthanide ion and labeled C3 as low as 5 x 10-10mol/liter could be detected. This protein chelator system has potential to be a useful, flexible complement to the organic chelators currently used in lanthanide-based, time-resolved luminescence immunoassays. © 1994 Academic Press, Inc. All rights reserved.
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页码:1 / 6
页数:6
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