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半乳糖血症诱导的培养晶状体上皮细胞中PGH合酶活性抑制的逆转。

Reversal of galactosemic-induced inhibition of PGH synthase activity in cultured lens epithelial cells.

作者信息

Cammarata P R, Jackson T, Lou M, Yorio T

机构信息

Department of Anatomy, Texas College of Osteopathic Medicine, Fort Worth, 76107.

出版信息

Curr Eye Res. 1989 Oct;8(10):1063-9. doi: 10.3109/02713688908997399.

Abstract

Inhibition of prostaglandin synthesis as determined by prostaglandin endoperoxide synthetase (PGH synthase) activity is associated with polyol accumulation in cultured bovine lens epithelial cells (BLECs) incubated six days in minimal essential medium (MEM) containing 40 mM galactose (Gal). In order to better understand the nature of the correlation between hypergalactosemic exposure, polyol accumulation and inhibition of prostaglandin synthesis, a series of culture media reversal and sorbinil (an aldose reductase inhibitor) addition studies were carried out. BLECs were incubated in Gal for six days, then changed to galactose-free MEM +/- sorbinil for a three day recovery period. PGH synthase activity reduced to 66% of control after six days of exposure to Gal. The simultaneous administration of sorbinil during a nine day Gal incubation significantly protected the enzymatic activity, while the activity of PGH synthase further declined to 41% of control under the same conditions in the absence of sorbinil. Within 72 hours of media reversal, PGH synthase activity equaled or exceeded control values in BLECs switched to either MEM or MEM + sorbinil. Indeed, an enhanced prostaglandin biosynthetic capacity as demonstrated by radioimmunoassay was exhibited with microsomes prepared from cells switched from Gal into Gal-free MEM +/- sorbinil, corroborating the beneficial effect of media reversal. Furthermore, following 72 hours of reversal, the cellular dulcitol level was 93 nmol/micrograms PO4 for BLECs switched to MEM alone; no detectable level of polyol was observed in BLECs changed to MEM + sorbinil. In contrast, the polyol content in BLECs after six days of exposure to Gal was 185 nmol/micrograms PO4 and increased to 334 nmol/micrograms PO4 after nine days of continuous incubation.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

通过前列腺素内过氧化物合成酶(PGH合成酶)活性测定的前列腺素合成抑制与在含有40 mM半乳糖(Gal)的最低限度基本培养基(MEM)中培养6天的培养牛晶状体上皮细胞(BLEC)中的多元醇积累有关。为了更好地理解高半乳糖血症暴露、多元醇积累和前列腺素合成抑制之间相关性的本质,进行了一系列培养基逆转和添加索比尼尔(一种醛糖还原酶抑制剂)的研究。BLEC在Gal中培养6天,然后换成不含半乳糖的MEM ± 索比尼尔,进行为期3天的恢复期。暴露于Gal 6天后,PGH合成酶活性降至对照的66%。在9天的Gal孵育期间同时给予索比尼尔可显著保护酶活性,而在相同条件下且无索比尼尔时,PGH合成酶活性进一步降至对照的41%。在培养基逆转的72小时内,切换到MEM或MEM + 索比尼尔的BLEC中PGH合成酶活性等于或超过对照值。实际上,从Gal换成不含半乳糖的MEM ± 索比尼尔的细胞制备的微粒体通过放射免疫测定显示出增强的前列腺素生物合成能力,证实了培养基逆转的有益效果。此外,逆转72小时后,切换到单独MEM的BLEC的细胞山梨醇水平为93 nmol/μg PO4;切换到MEM + 索比尼尔的BLEC中未观察到可检测水平的多元醇。相比之下,暴露于Gal 6天后BLEC中的多元醇含量为185 nmol/μg PO4,连续孵育9天后增加至334 nmol/μg PO4。(摘要截短于250字)

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