Halio S B, Blumentals I I, Short S A, Merrill B M, Kelly R M
Department of Chemical Engineering, North Carolina State University, Raleigh, 27695-7905, USA.
J Bacteriol. 1996 May;178(9):2605-12. doi: 10.1128/jb.178.9.2605-2612.1996.
A previously identified intracellular proteolytic activity in the hyperthermophilic archaeon Pyrococcus furiosus (I. I. Blumentals, A. S. Robinson, and R. M. Kelly, Appl. Environ. Microbiol. 56:1992-1998, 1990) was found to be a homomultimer consisting of 18.8-kDa subunits. Dissociation of this native P. furiosus protease I (PfpI) into a single subunit was seen by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) but only after trichloroacetic acid precipitation; heating to 95 degrees C in the presence of 2% SDS and 80 mM dithiothreitol did not dissociate the protein. The gene (pfpI) coding for this protease was located in genomic digests by Southern blotting with probes derived from the N-terminal amino acid sequence. pfpI was cloned, sequenced, and expressed in active form in Escherichia coli as a fusion protein with a histidine tag. The recombinant protease from E. coli showed maximum proteolytic activity at 95 degrees C, and its half-life was 19 min at this temperature. This level of stability was significantly below that previously reported for the enzyme purified by electroelution of a 66-kDa band from SDS-PAGE after extended incubation of cell extracts at 98 degrees C in 1% SDS (>30 h). The pfpI gene codes for a polypeptide of 166 amino acid residues lacking any conserved protease motifs; no protease activity was detected for the 18.8-kDa PfpI subunit (native or recombinant) by substrate gel assay. Although an immunological relationship of this protease to the eukaryotic proteasome has been seen previously, searches of the available databases identified only two similar amino acid sequences: an open reading frame of unknown function from Staphylococcus aureus NCTC 8325 (171 amino acid residues, 18.6 kDa, 41% identity) and an open reading frame also of unknown function in E. coli (172 amino acid residues, 18.8 kDa, 47% identity). Primer extension experiments with P. furiosus total RNA defined the 5' end of the transcript. There are only 10 nucleotides upstream of the start of translation; therefore, it is unlikely that there are any pre- or pro-regions associated with PfpI which could have been used for targeting or assembly of this protease. Although PfpI activity appears to be the dominant proteolytic activity in P. furiosus cell extracts, the physiological function of PfpI is unclear.
先前在嗜热古菌激烈火球菌(I. I. 布卢门塔尔斯、A. S. 罗宾逊和R. M. 凯利,《应用与环境微生物学》56:1992 - 1998,1990年)中鉴定出的一种细胞内蛋白水解活性被发现是一种由18.8 kDa亚基组成的同多聚体。通过十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳(SDS - PAGE)观察到这种天然的激烈火球菌蛋白酶I(PfpI)解离为单个亚基,但这仅在三氯乙酸沉淀后才出现;在2% SDS和80 mM二硫苏糖醇存在下加热至95℃并不能使该蛋白解离。通过用源自N端氨基酸序列的探针进行Southern印迹分析,在基因组消化物中定位了编码这种蛋白酶的基因(pfpI)。pfpI被克隆、测序,并作为带有组氨酸标签的融合蛋白在大肠杆菌中以活性形式表达。来自大肠杆菌的重组蛋白酶在95℃时显示出最大蛋白水解活性,并且在该温度下其半衰期为19分钟。这种稳定性水平明显低于先前报道的通过在1% SDS中于98℃对细胞提取物进行长时间孵育(>30小时)后从SDS - PAGE中电洗脱66 kDa条带而纯化得到的酶的稳定性。pfpI基因编码一个由166个氨基酸残基组成的多肽,缺乏任何保守的蛋白酶基序;通过底物凝胶分析未检测到18.8 kDa的PfpI亚基(天然的或重组的)具有蛋白酶活性。尽管先前已经观察到这种蛋白酶与真核蛋白酶体存在免疫关系,但在可用数据库中搜索仅发现两个相似的氨基酸序列:来自金黄色葡萄球菌NCTC 8325的一个功能未知的开放阅读框(171个氨基酸残基,18.6 kDa,41% 同一性)和大肠杆菌中一个同样功能未知的开放阅读框(172个氨基酸残基,18.8 kDa,47% 同一性)。用激烈火球菌总RNA进行的引物延伸实验确定了转录本的5' 端。翻译起始位点上游仅10个核苷酸;因此,不太可能存在与PfpI相关的任何前体或原区域可用于该蛋白酶的靶向或组装。尽管PfpI活性似乎是激烈火球菌细胞提取物中的主要蛋白水解活性,但PfpI的生理功能尚不清楚。
