Pseudomonas aeruginosa peptide peptidohydrolase

Kazuyuki Morihasa, Hiroshige Tsuzuki
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引用次数: 24

Abstract

The twice recrystallized proteinase (peptide peptidohydrolase) of Pseudomonas aeruginosa IFO 3080 contained 1–2 gramatoms of Ca per mole (48 400 g) of enzyme protein and insignificant amounts of the other metal ions. Some chelating agents, such as ethylenediaminetetraacetic acid and o-phenanthroline, inhibited the enzymic activity, but the inactivation at 40° or below was easily reversed either by dialysis, dilution or the addition of various metal ions such as Zn2+, Co2+, Ca2+, etc. The Ca content of the enzyme protein was not decreased by the reversible inactivation, showing that the inactivation was produced by masking the Ca2+ of the enzyme with the chelating agent. To dissociate the Ca2+ from the enzyme protein, the inactivation treatment by chelating agent was made at 50°, but the trial was unsuccessful, that is, reactivation was no longer observed during the autodigestion of the enzyme protein. Thus the proteinase was regarded as a Ca2+-metalloenzyme, in which Ca2+ was tightly bound to the enzyme protein.

铜绿假单胞菌IFO 3080的二次重结晶蛋白酶(肽肽水解酶)每摩尔(48 400 g)含有1-2克Ca,其他金属离子含量不高。一些螯合剂,如乙二胺四乙酸和邻菲罗啉,抑制酶的活性,但在40°或以下的失活很容易通过透析、稀释或添加各种金属离子如Zn2+、Co2+、Ca2+等来逆转。酶蛋白的钙含量不因可逆失活而降低,说明失活是通过螯合剂掩盖酶的Ca2+而产生的。为了将Ca2+从酶蛋白上解离,在50°下进行了螯合剂失活处理,但试验失败,即酶蛋白自消化过程中不再观察到再活化。因此,蛋白酶被认为是一种Ca2+-金属酶,其中Ca2+与酶蛋白紧密结合。
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