首页> 外文期刊>Journal of bacteriology >Bacillus subtilis HemY is a peripheral membrane protein essential for protoheme IX synthesis which can oxidize coproporphyrinogen III and protoporphyrinogen IX.
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Bacillus subtilis HemY is a peripheral membrane protein essential for protoheme IX synthesis which can oxidize coproporphyrinogen III and protoporphyrinogen IX.

机译:枯草芽孢杆菌HemY是原血红素IX合成必不可少的外围膜蛋白,它可以氧化原卟啉原III和原卟啉原IX。

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The hemY gene of the Bacillus subtilis hemEHY operon is essential for protoheme IX biosynthesis. Two previously isolated hemY mutations were sequenced. Both mutations are deletions affecting the hemY reading frame, and they cause the accumulation of coproporphyrinogen III or coproporphyrin III in the growth medium and the accumulation of trace amounts of other porphyrinogens or porphyrins intracellularly. HemY was found to be a 53-kDa peripheral membrane-bound protein. In agreement with recent findings by Dailey et al. (J. Biol. Chem. 269:813-815, 1994) B. subtilis HemY protein synthesized in Escherichia coli oxidized coproporphyrinogen III and protoporphyrinogen IX to coproporphyrin and protoporphyrin, respectively. The protein is not a general porphyrinogen oxidase since it did not oxidize uroporphyrinogen III. The apparent specificity constant, kcat/Km, for HemY was found to be about 12-fold higher with coproporphyrinogen III as a substrate compared with protoporphyrinogen IX as a substrate. The protoporphyrinogen IX oxidase activity is consistent with the function of HemY in a late step of protoheme IX biosynthesis, i.e., HemY catalyzes the penultimate step of the pathway. However, the efficient coproporphyrinogen III to coproporphyrin oxidase activity is unexplained in the current view of protoheme IX biosynthesis.
机译:枯草芽孢杆菌hemEHY操纵子的hemY基因对于原血红素IX生物合成至关重要。对两个先前分离的hemY突变进行测序。两种突变都是影响hemY阅读框的缺失,并且它们导致辅卟啉原III或辅卟啉III在生长培养基中的积累以及细胞内痕量其他卟啉原或卟啉的积累。发现HemY是53kDa外周膜结合蛋白。与Dailey等人的最新发现一致。 (J. Biol。Chem。269:813-815,1994)在大肠杆菌中合成的枯草芽孢杆菌HemY蛋白将氧化原卟啉原III和原卟啉原IX分别氧化为原卟啉和原卟啉。该蛋白质不是一般的卟啉原氧化酶,因为它不氧化尿卟啉原III。发现与原卟啉原IX作为底物相比,以辅卟啉原原III作为底物,对HemY的表观特异性常数kcat / Km高约12倍。原卟啉原IX氧化酶的活性与原血红素IX生物合成的后期步骤中的HemY的功能一致,即HemY催化该途径的倒数第二步。然而,在原血红素IX生物合成的当前观点中,无法解释有效的原卟啉原III对原卟啉氧化酶的活性。

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