Wu L F, Mandrand M A
Laboratoire de Génétique Moléculaire des Microorganismes, CNRS URA 1486, INSA, Villeurbanne, France.
FEMS Microbiol Rev. 1993 Apr;10(3-4):243-69. doi: 10.1111/j.1574-6968.1993.tb05870.x.
Thirty sequenced microbial hydrogenases are classified into six classes according to sequence homologies, metal content and physiological function. The first class contains nine H2-uptake membrane-bound NiFe-hydrogenases from eight aerobic, facultative anaerobic and anaerobic bacteria. The second comprises four periplasmic and two membrane-bound H2-uptake NiFe(Se)-hydrogenases from sulphate-reducing bacteria. The third consists of four periplasmic Fe-hydrogenases from strict anaerobic bacteria. The fourth contains eight methyl-viologen- (MV), factor F420- (F420) or NAD-reducing soluble hydrogenases from methanobacteria and Alcaligenes eutrophusH16. The fifth is the H2-producing labile hydrogenase isoenzyme 3 of Escherichia coli. The sixth class contains two soluble tritium-exchange hydrogenases of cyanobacteria. The results of sequence comparison reveal that the 30 hydrogenases have evolved from at least three different ancestors. While those of class I, II, IV and V hydrogenases are homologous, i.e. sharing the same evolutionary origin, both class III and VI hydrogenases are neither related to each other nor to the other classes. Sequence comparison scores, hierarchical cluster structures and phylogenetic trees show that class II falls into two distinct clusters composed of NiFe- and NiFeSe-hydrogenases, respectively. These results also reveal that class IV comprises three distinct clusters: MV-reducing, F420-reducing and NAD-reducing hydrogenases. Specific signatures of the six classes of hydrogenases as well as some subclusters have been detected. Analyses of motif compositions indicate that all hydrogenases, except those of class VI, must contain some common motifs probably participating in the formation of hydrogen activation domains and electron transfer domains. The regions of hydrogen activation domains are highly conserved and can be divided into two categories. One corresponds to the 'nickel active center' of NiFe(Se)-hydrogenases. It consists of two possible specific nickel-binding motifs, RxCGxCxxxH and DPCxxCxxH, located at the N- and C-termini of so-called large subunits in the dimeric hydrogenases, respectively. The other is the H-cluster of the Fe-hydrogenases. It might comprise three motifs on the C-terminal half of the large subunits. However, the motifs corresponding to the putative electron transfer domains, as well as their polypeptides chains, are poorly or even not at all conserved. They are present essentially on the small subunits in NiFe-hydrogenases. Some of these motifs resemble the typical ferredoxin-like Fe-S cluster binding site.(ABSTRACT TRUNCATED AT 400 WORDS)
根据序列同源性、金属含量和生理功能,30种已测序的微生物氢化酶被分为六类。第一类包含来自8种好氧、兼性厌氧和厌氧细菌的9种膜结合型摄取氢气的镍铁氢化酶。第二类包括来自硫酸盐还原菌的4种周质型和2种膜结合型摄取氢气的镍铁(硒)氢化酶。第三类由来自严格厌氧细菌的4种周质型铁氢化酶组成。第四类包含来自甲烷杆菌和嗜碱产碱菌H16的8种甲基紫精(MV)、F420或NAD还原型可溶性氢化酶。第五类是大肠杆菌产生氢气的不稳定氢化酶同工酶3。第六类包含蓝细菌的2种可溶性氚交换氢化酶。序列比较结果表明,这30种氢化酶至少从3个不同的祖先进化而来。第一、二、四和五类氢化酶具有同源性,即具有相同的进化起源,而第三类和第六类氢化酶彼此之间以及与其他类均无关联。序列比较得分、层次聚类结构和系统发育树表明,第二类分为两个不同的簇,分别由镍铁氢化酶和镍铁硒氢化酶组成。这些结果还表明,第四类包括三个不同的簇:MV还原型、F420还原型和NAD还原型氢化酶。已检测到六类氢化酶以及一些亚簇的特定特征。基序组成分析表明,除第六类外,所有氢化酶都必须包含一些可能参与氢激活域和电子传递域形成的共同基序。氢激活域区域高度保守,可分为两类。一类对应于镍铁(硒)氢化酶的“镍活性中心”。它由两个可能的特定镍结合基序RxCGxCxxxH和DPCxxCxxH组成,分别位于二聚体氢化酶中所谓大亚基的N端和C端。另一类是铁氢化酶的H簇。它可能在大亚基的C端一半包含三个基序。然而,对应于假定电子传递域的基序及其多肽链保守性较差甚至根本不保守。它们主要存在于镍铁氢化酶的小亚基上。其中一些基序类似于典型的铁氧化还原蛋白样铁硫簇结合位点。(摘要截短于400字)
