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细胞色素P - 450系统介导的溴苯对大鼠δ-氨基乙酰丙酸脱水酶活性的抑制作用

Cytochrome P-450 system dependent depression of delta-aminolevulinic acid dehydratase activity by bromobenzene in rats.

作者信息

Koizumi A, Fujita H, Sadamoto T, Ohmachi T, Watanabe M, Ikeda M

出版信息

Toxicology. 1984 Jul;32(1):1-10. doi: 10.1016/0300-483x(84)90029-5.

Abstract

Male Wistar rats (200-230 g) were treated with bromobenzene in soybean oil intraperitoneally (i.p.) (4 mmol/kg) once a day for 1 or 2 days while control rats received soybean oil alone. delta-Aminolevulinic acid dehydratase (ALA-D) activity was depressed to 80% and 43% in bone marrow after 24 h and 48 h, respectively. ALA-D activity was also depressed significantly in the liver after the administration of bromobenzene while the activity in peripheral erythrocytes was not altered. After the administration of bromobenzene, the concentration of reduced non-protein sulfhydryls in liver was the lowest at 24 h and increased thereafter. No significant change was observed in the activity of delta-aminolevulinate synthase in liver. The decrease of ALA-D activity was also reproducible in vitro. The 105 000 g supernatant fractions of rat bone marrow lyzates as ALA-D source were incubated with liver microsomes prepared from rats treated with phenobarbital. ALA-D activity was decreased by bromobenzene but no decrease was observed when the microsomes were preincubated with CO to inhibit cytochrome P-450. The effect of bromobenzene on ALA-D purified from rat erythroid cells was studied in incubations containing a reconstituted cytochrome P-450 system prepared from rat liver. The decrease of ALA-D activity was proportional to both the incubation time and to the concentration of P-450 while no decrease was detected when P-450 was inhibited by CO before the incubation.

摘要

雄性Wistar大鼠(200 - 230克)腹腔注射(i.p.)溶于大豆油中的溴苯(4毫摩尔/千克),每天一次,持续1或2天,而对照大鼠仅接受大豆油。24小时和48小时后,骨髓中的δ-氨基乙酰丙酸脱水酶(ALA-D)活性分别降至80%和43%。给予溴苯后,肝脏中的ALA-D活性也显著降低,而外周红细胞中的活性未改变。给予溴苯后,肝脏中还原型非蛋白巯基的浓度在24小时时最低,此后升高。肝脏中δ-氨基乙酰丙酸合酶的活性未观察到显著变化。ALA-D活性的降低在体外也可重现。将大鼠骨髓裂解物的105000克上清液组分作为ALA-D来源,与用苯巴比妥处理的大鼠制备的肝微粒体一起孵育。溴苯可降低ALA-D活性,但当微粒体预先用CO孵育以抑制细胞色素P - 450时,未观察到活性降低。在含有从大鼠肝脏制备的重组细胞色素P - 450系统的孵育中,研究了溴苯对从大鼠红系细胞纯化的ALA-D的影响。ALA-D活性的降低与孵育时间和P - 450浓度均成正比,而在孵育前用CO抑制P - 450时未检测到活性降低。

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