Wilson H L, Aldrich H C, Maupin-Furlow J
Department of Microbiology and Cell Science, University of Florida, Gainesville, Florida 32611-0700, USA.
J Bacteriol. 1999 Sep;181(18):5814-24. doi: 10.1128/JB.181.18.5814-5824.1999.
A 20S proteasome, composed of alpha(1) and beta subunits arranged in a barrel-shaped structure of four stacked rings, was purified from a halophilic archaeon Haloferax volcanii. The predominant peptide-hydrolyzing activity of the 600-kDa alpha(1)beta-proteasome on synthetic substrates was cleavage carboxyl to hydrophobic residues (chymotrypsin-like [CL] activity) and was optimal at 2 M NaCl, pH 7.7 to 9.5, and 75 degrees C. The alpha(1)beta-proteasome also hydrolyzed insulin B-chain protein. Removal of NaCl inactivated the CL activity of the alpha(1)beta-proteasome and dissociated the complex into monomers. Rapid equilibration of the monomers into buffer containing 2 M NaCl facilitated their reassociation into fully active alpha(1)beta-proteasomes of 600 kDa. However, long-term incubation of the halophilic proteasome in the absence of salt resulted in hydrolysis and irreversible inactivation of the enzyme. Thus, the isolated proteasome has unusual salt requirements which distinguish it from any proteasome which has been described. Comparison of the beta-subunit protein sequence with the sequence deduced from the gene revealed that a 49-residue propeptide is removed to expose a highly conserved N-terminal threonine which is proposed to serve as the catalytic nucleophile and primary proton acceptor during peptide bond hydrolysis. Consistent with this mechanism, the known proteasome inhibitors carbobenzoxyl-leucinyl-leucinyl-leucinal-H (MG132) and N-acetyl-leucinyl-leucinyl-norleucinal (calpain inhibitor I) were found to inhibit the CL activity of the H. volcanii proteasome (K(i) = 0.2 and 8 microM, respectively). In addition to the genes encoding the alpha(1) and beta subunits, a gene encoding a second alpha-type proteasome protein (alpha(2)) was identified. All three genes coding for the proteasome subunits were mapped in the chromosome and found to be unlinked. Modification of the methods used to purify the alpha(1)beta-proteasome resulted in the copurification of the alpha(2) protein with the alpha(1) and beta subunits in nonstoichometric ratios as cylindrical particles of four stacked rings of 600 kDa with CL activity rates similar to the alpha(1)beta-proteasome, suggesting that at least two separate 20S proteasomes are synthesized. This study is the first description of a prokaryote which produces two separate 20S proteasomes and suggests that there may be distinct physiological roles for the two different alpha subunits in this halophilic archaeon.
从嗜盐古菌沃氏嗜盐菌(Haloferax volcanii)中纯化出一种20S蛋白酶体,它由α(1)和β亚基组成,排列成四个堆叠环的桶状结构。600 kDa的α(1)β-蛋白酶体对合成底物的主要肽水解活性是在疏水性残基的羧基端进行切割(类胰凝乳蛋白酶样[CL]活性),在2 M NaCl、pH 7.7至9.5和75℃条件下活性最佳。α(1)β-蛋白酶体也能水解胰岛素B链蛋白。去除NaCl会使α(1)β-蛋白酶体的CL活性失活,并使复合物解离成单体。单体快速平衡到含有2 M NaCl的缓冲液中有助于它们重新结合成600 kDa的完全活性的α(1)β-蛋白酶体。然而,嗜盐蛋白酶体在无盐条件下长期孵育会导致酶的水解和不可逆失活。因此,分离出的蛋白酶体有不同寻常的盐需求,这使其与已描述的任何蛋白酶体都不同。将β亚基的蛋白质序列与从基因推导的序列进行比较,发现一个49个残基的前肽被去除,暴露出一个高度保守的N端苏氨酸,该苏氨酸被认为在肽键水解过程中作为催化亲核试剂和主要质子受体。与这种机制一致,已知的蛋白酶体抑制剂苄氧羰基-亮氨酰-亮氨酰-亮氨醛-H(MG132)和N-乙酰-亮氨酰-亮氨酰-正亮氨醛(钙蛋白酶抑制剂I)被发现可抑制沃氏嗜盐菌蛋白酶体的CL活性(K(i)分别为0.2和8 μM)。除了编码α(1)和β亚基的基因外,还鉴定出一个编码第二种α型蛋白酶体蛋白(α(2))的基因。编码蛋白酶体亚基的所有三个基因都定位在染色体上,并且发现它们是不连锁的。对用于纯化α(1)β-蛋白酶体的方法进行改进,导致α(2)蛋白与α(1)和β亚基以非化学计量比共纯化,形成四个堆叠环的600 kDa圆柱形颗粒,其CL活性速率与α(1)β-蛋白酶体相似,这表明至少合成了两种不同的20S蛋白酶体。这项研究首次描述了一种产生两种不同20S蛋白酶体的原核生物,并表明在这种嗜盐古菌中,两种不同的α亚基可能有不同的生理作用。
