Chang H C, Holland R D, Bumpus J A, Churchwell M I, Doerge D R
Division of Biochemical Toxicology, National Center for Toxicological Research, FDA, Jefferson, AR 72079, USA.
Chem Biol Interact. 1999 Dec 15;123(3):197-217. doi: 10.1016/s0009-2797(99)00136-2.
The peroxidase from Coprinus cinereus (CPX) catalyzed oxidative oligomerization of 4-chloroaniline (4-CA) forming several products: N-(4-chlorophenyl)-benzoquinone monoamine (dimer D), 4,4'-dichloroazobenzene (dimer E); 2-(4-chloroanilino)-N-(4-chlorophenyl)-benzoquinone (trimer F); 2-amino-5-chlorobenzoquinone-di-4-chloroanil (trimer G); 2-(4-chloroanilino)-5-hydroxybenzoquinone-di-4-chloroanil (tetramer H) and 2-amino-5-(-4-chlroanilino)-benzoquinone-di-4-chloroanil (tetramer 1). In the presence of 4-CA and H2O2, CPX was irreversibly inactivated within 10 min. Inactivation of CPX in the presence of H2O2 was a time-dependent, first-order process when the concentration of 4-CA was varied between 0 and 2.5 mM. The apparent dissociation constant (Ki) for CPX and 4-CA was 0.71 mM. The pseudo-first order rate constant for inactivation (k(inact)), was 1.15 x 10(-2) s(-1). Covalent incorporation of 20 mole 14C-4-CA per mole of inactivated CPX was observed. The partition ratio was about 2200 when either 4-CA or H2O2 was used as the limiting substrate. These results show that 4-CA is a metabolically activated inactivator (i.e. a suicide substrate). Unmodified heme and hydroxymethyl heme were isolated from native, 4-CA-inactivated and H2O2-incubated CPX. Inactivation resulted in significant losses in both heme contents. Analysis of tryptic peptides from 4-CA-inactivated CPX by MALDI-TOF/ MS and UV-VIS spectrophotometry suggested that trimer G and tetramer H were the major 4-CA derivatives that were covalently bound, including to a peptide (MGDAGF-SPDEVVDLLAAHSLASQEGLNSAIFR) containing the heme binding site. These studies show that heme destruction and covalent modification of the polypeptide chain are both important for the inactivation of CPX. These results were compared with similar studies on 4-CA-inactivated horseradish peroxidase (HRP) and bovine lactoperoxidase (LPO) during the oxidation of 4-CA.
灰盖鬼伞过氧化物酶(CPX)催化4-氯苯胺(4-CA)发生氧化寡聚反应,生成多种产物:N-(4-氯苯基)-苯醌单胺(二聚体D)、4,4'-二氯偶氮苯(二聚体E);2-(4-氯苯胺基)-N-(4-氯苯基)-苯醌(三聚体F);2-氨基-5-氯苯醌-二-4-氯苯胺(三聚体G);2-(4-氯苯胺基)-5-羟基苯醌-二-4-氯苯胺(四聚体H)和2-氨基-5-(-4-氯苯胺基)-苯醌-二-4-氯苯胺(四聚体I)。在4-CA和H2O2存在的情况下,CPX在10分钟内不可逆地失活。当4-CA的浓度在0至2.5 mM之间变化时,H2O2存在下CPX的失活是一个时间依赖性的一级过程。CPX与4-CA的表观解离常数(Ki)为0.71 mM。失活的伪一级速率常数(k(inact))为1.15×10(-2)s(-1)。观察到每摩尔失活的CPX共价结合20摩尔14C-4-CA。当以4-CA或H2O2作为限制底物时,分配比约为2200。这些结果表明4-CA是一种代谢活化的失活剂(即自杀底物)。从未修饰的血红素和羟甲基血红素分别从天然的、4-CA失活的和H2O2孵育的CPX中分离出来。失活导致血红素含量显著损失。通过基质辅助激光解吸电离飞行时间质谱(MALDI-TOF/MS)和紫外可见分光光度法对4-CA失活的CPX的胰蛋白酶肽段进行分析表明,三聚体G和四聚体H是主要的共价结合的4-CA衍生物,包括与一个含有血红素结合位点的肽段(MGDAGF-SPDEVVDLLAAHSLASQEGLNSAIFR)结合。这些研究表明,血红素破坏和多肽链的共价修饰对CPX的失活都很重要。将这些结果与4-CA氧化过程中4-CA失活的辣根过氧化物酶(HRP)和牛乳铁过氧化物酶(LPO)的类似研究进行了比较。
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