IN-VITRO SYNTHESIS OF THE IRON-MOLYBDENUM COFACTOR OF NITROGENASE - PURIFICATION AND CHARACTERIZATION OF NIFB COFACTOR, THE PRODUCT OF NIFB PROTEIN

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作者
SHAH, VK
ALLEN, JR
SPANGLER, NJ
LUDDEN, PW
机构
[1] UNIV WISCONSIN,COLL AGR & LIFE SCI,DEPT BIOCHEM,MADISON,WI 53706
[2] UNIV WISCONSIN,COLL AGR & LIFE SCI,CTR STUDIES NITROGEN FIXAT,MADISON,WI 53706
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中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The requirement of NIFB activity for the biosynthesis of iron-molybedenum cofactor (FeMo-co) can be satisfied by the addition of the low molecular weight product of NIFB, termed NifB cofactor (NifB-co). NifB-co has been purified to homogeneity by a unique one-step method. Addition of NifB-co into the FeMo-co synthesis system generated nitrogenase activity of 27-32 nmol of ethylene formed/min/nmol of iron. Iron is the only metal detected in the NifB-co. NifB-co-dependent in vitro FeMo-co synthesis is absolutely dependent on the presence of molybdate, homocitrate and active NIFNE protein in the reaction mixture. The cofactor appears to be a small Fe-S cluster synthesized by NIFB, as a precursor of FeMo-co. NifB-co did not display any EPR signal at 4 K in 0-4000 gauss range. A solution of NifB-co is greenish-brown in color, similar to FeMo-co. NifB-co exhibits a broad absorbance between 400 and 700 nm with no distinctive peaks or shoulders. NifB-co is stable to repeated freeze-thaw cycles and is also stable in N-methylformamide, the solvent used for the isolation of FeMo-co. The NifB-co is stable to a 5-min heat treatment at 60-degrees-C. The cofactor is extremely O2-labile, with half-life of less then 15 s in air.
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页码:1154 / 1158
页数:5
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