齿垢密螺旋体ATCC 35405中类胰凝乳蛋白酶样膜相关蛋白酶在生物活性肽失活中的作用
Role of the chymotrypsin-like membrane-associated proteinase from Treponema denticola ATCC 35405 in inactivation of bioactive peptides.
作者信息
Mäkinen P L, Mäkinen K K, Syed S A
机构信息
Department of Biologic and Materials Sciences, School of Dentistry, University of Michigan, Ann Arbor 48109, USA.
出版信息
Infect Immun. 1995 Sep;63(9):3567-75. doi: 10.1128/iai.63.9.3567-3575.1995.
The ability of washed whole cells of Treponema denticola ATCC 35405 to hydrolyze (inactivate) substance P, bradykinin, and angiotensin I was studied. Substance P was attacked primarily at the Phe-8-Gly-9 bond by a chymotrypsin-like proteinase (CTLP), at Pro-4-Gln-5 by an endo-acting prolyl oligopeptidase (POPase), and at Gln-5-Gln-6 by an endopeptidase (FALGPA-peptidase). Bradykinin was cleaved at Phe-5-Ser-6 by the FALGPA-peptidase and at Pro-7-Phe-8 by the POPase. Angiotensin I was rapidly converted to angiotensin II by the CTLP, and both angiotensin I and angiotensin II were further hydrolyzed at Pro-7-Phe-8 by the POPase. All these enzymes were assumed to be cell associated and were easily extracted with a mild (0.05 to 0.1%) Triton X-100 treatment. Because it was conceivable that the hydrolysis of substance P at the Phe-8-Gly-9 bond was catalyzed by a CTLP described earlier (V.-J. Uitto, D. Grenier, E. C. S. Chan, and B. C. McBride, Infect. Immun. 56:2717-2722, 1988), the enzyme was purified to homogeneity by means of conventional fast protein liquid chromatography procedures. For kinetic studies, Phe-8(4-nitro)-substance P (NSP) (absorption maximum at 309.2 nm, epsilon = 545 M-1 cm-1) was synthesized to replace substance P as a substrate in kinetic studies. In reversed-phase chromatography, both NSP and substance P gave identical results with both whole cells and the purified enzyme. The CTLP has a mass of 95 kDa, and its activity is suggested to be based on an active seryl residue, on an active imidazole group, and on an active carboxyl group but not on metal cations. The enzyme hydrolyzes N-succinyl-L-Ala-L-Ala-L-Pro-L-Phe-p-nitroaniline (SAAPFNA, a typical chymotrypsin substrate) at a high rate and several proteins, such as calf thymus histone, human plasma fibrinogen, milk caseins, and gelatin. Among the substrates tested, substance P showed the highest affinity (Km = 0.22 mM) for the purified enzyme. Depending on conditions, clinically applicable chlorhexidine levels (3.2 mmol/liter, or 0.2%) strongly activated (up to fourfold) the hydrolysis of SAAPFNA by whole cells and the purified CTLP. The hydrolysis of NSP by whole cells and purified CTLP was slightly inhibited by chlorhexidine. The results demonstrated the versatility and the effectiveness of the outer membrane of T. denticola in occasioning a rapid breakdown and inactivation of human bioactive peptides and other peptidolytic catalyses.(ABSTRACT TRUNCATED AT 400 WORDS)
研究了具核梭杆菌ATCC 35405的洗涤全细胞水解(灭活)P物质、缓激肽和血管紧张素I的能力。P物质主要被一种类胰凝乳蛋白酶(CTLP)作用于Phe-8-Gly-9键,被一种内切脯氨酰寡肽酶(POPase)作用于Pro-4-Gln-5键,被一种内肽酶(FALGPA-肽酶)作用于Gln-5-Gln-6键。缓激肽被FALGPA-肽酶作用于Phe-5-Ser-6键,被POPase作用于Pro-7-Phe-8键。血管紧张素I被CTLP迅速转化为血管紧张素II,血管紧张素I和血管紧张素II都被POPase进一步作用于Pro-7-Phe-8键。所有这些酶都被认为与细胞相关,并且用温和的(0.05%至0.1%) Triton X-100处理很容易提取出来。因为可以想象P物质在Phe-8-Gly-9键处的水解是由先前描述的一种CTLP催化的(V.-J. Uitto、D. Grenier、E. C. S. Chan和B. C. McBride,《感染与免疫》56:2717 - 2722,1988),所以通过常规的快速蛋白质液相色谱程序将该酶纯化至同质。为了进行动力学研究,合成了Phe-8(4-硝基)-P物质(NSP)(在309.2 nm处有最大吸收,ε = 545 M-1 cm-1)以替代P物质作为动力学研究中的底物。在反相色谱中,NSP和P物质在全细胞和纯化酶中都给出了相同的结果。CTLP的质量为95 kDa,其活性被认为基于一个活性丝氨酰残基、一个活性咪唑基团和一个活性羧基,而不是基于金属阳离子。该酶能高速水解N-琥珀酰-L-丙氨酸-L-丙氨酸-L-脯氨酸-L-苯丙氨酸-对硝基苯胺(SAAPFNA,一种典型的胰凝乳蛋白酶底物)以及几种蛋白质,如小牛胸腺组蛋白、人血浆纤维蛋白原、牛奶酪蛋白和明胶。在所测试的底物中,P物质对纯化酶显示出最高的亲和力(Km = 0.22 mM)。根据条件,临床适用的洗必泰水平(3.2 mmol/升,或0.2%)能强烈激活(高达四倍)全细胞和纯化的CTLP对SAAPFNA的水解。洗必泰对全细胞和纯化的CTLP水解NSP有轻微抑制作用。结果证明了具核梭杆菌外膜在促使人类生物活性肽快速分解和失活以及其他肽水解催化方面的多功能性和有效性。(摘要截短至400字)
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