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Evidence that cysteine-166 is the active-site nucleophile of Pseudomonas aeruginosa amidase: crystallization and preliminary X-ray diffraction analysis of the enzyme.

机译:半胱氨酸166是铜绿假单胞菌酰胺酶活性位点亲核试剂的证据:该酶的结晶和初步X射线衍射分析。

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摘要

Wild-type and site-specific mutants C166S and C166A (Cys-166-->Ser and Cys-166-->Ala respectively) of the amidase (acylamide amidohydrolase, EC 3.5.1.4) from Pseudomonas aeruginosa were expressed in Escherichia coli by using the vector pKK223-3. Both mutant proteins were catalytically inactive but showed complete cross-reactivity with polyclonal antiserum raised against the wild-type enzyme, as well as CD spectra identical with that of the wild-type enzyme, which were indicative of correct folding. Cys-166 is therefore implicated as the active-site nucleophile. Titration of free thiol groups with 5,5'-dithiobis-(2-nitrobenzoic acid) indicated that Cys-166 is not a rapidly reacting residue. Crystals of both wild-type and C166S amidase grew with identical, rhombohedral morphology; X-ray diffraction analysis established the unit cell dimensions (a=b=c=84 A; alpha=beta=gamma=75 degrees) and space group (R3 or R32). These results imply a quaternary structure of six subunits, with most probably 32 symmetry; the existence of a hexameric structure was supported by molecular mass determinations based on gel filtration and electrophoretic mobility.
机译:来自铜绿假单胞菌的酰胺酶(酰胺酰胺水解酶,EC 3.5.1.4)的野生型和位点特异性突变体C166S和C166A(分别为Cys-166-> Ser和Cys-166-> Ala)在大肠杆菌中表达使用载体pKK223-3。两种突变蛋白均无催化活性,但显示出与针对野生型酶的多克隆抗血清完全交叉的反应性,以及与野生型酶相同的CD光谱,表明正确的折叠。因此,Cys-166被认为是活性位点亲核试剂。用5,5'-二硫代双-(2-硝基苯甲酸)滴定游离硫醇基团表明Cys-166不是快速反应的残基。野生型和C166S酰胺酶的晶体均生长,具有相同的菱面体形态。 X射线衍射分析确定了晶胞尺寸(a = b = c = 84A;α=β=γ= 75度)和空间群(R3或R32)。这些结果暗示了六个亚基的四级结构,最可能具有32个对称性。基于凝胶过滤和电泳迁移率的分子量测定支持了六聚体结构的存在。

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