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组织蛋白酶A是催化抗逆转录病毒核苷酸膦酸酰胺前药GS-7340和GS-9131细胞内水解的主要水解酶。

Cathepsin A is the major hydrolase catalyzing the intracellular hydrolysis of the antiretroviral nucleotide phosphonoamidate prodrugs GS-7340 and GS-9131.

作者信息

Birkus Gabriel, Wang Ruth, Liu Xiaohong, Kutty Nilima, MacArthur Holly, Cihlar Tomas, Gibbs Craig, Swaminathan Swami, Lee William, McDermott Martin

机构信息

Gilead Sciences, Inc., 333 Lakeside Drive, Foster City, CA 94404, USA.

出版信息

Antimicrob Agents Chemother. 2007 Feb;51(2):543-50. doi: 10.1128/AAC.00968-06. Epub 2006 Dec 4.

Abstract

GS-7340 and GS-9131 {9-[(R)-2-[[(S)-[[(S)-1-(isopropoxycarbonyl)ethyl]amino]phenoxyphosphinyl]methoxy]-propyl]adenine and 9-(R)-4'-(R)-[[[(S)-1-[(ethoxycarbonyl)ethyl]amino]phenoxyphosphinyl]methoxy]-2'-fluoro-1'-furanyladenine, respectively} are novel alkylalaninyl phenyl ester prodrugs of tenofovir {9-R-[(2-phosphonomethoxy)propyl]adenine} (TFV) and a cyclic nucleotide analog, GS-9148 (phosphonomethoxy-2'-fluoro-2', 3'-dideoxydidehydroadenosine), respectively. Both prodrugs exhibit potent antiretroviral activity against both wild-type and drug-resistant human immunodeficiency virus type 1 strains and excellent in vivo pharmacokinetic properties. In this study, the main enzymatic activity responsible for the initial step in the intracellular activation of GS-7340 and GS-9131 was isolated from human peripheral blood mononuclear cells and identified as lysosomal carboxypeptidase A (cathepsin A [CatA]; EC 3.4.16.5). Biochemical properties of the purified hydrolase (native complex and catalytic subunit molecular masses of 100 and 29 kDa, respectively; isoelectric point [pI] of 5.5) matched those of CatA. Recombinant CatA and the isolated prodrug hydrolase displayed identical susceptibilities to inhibitors and identical substrate preferences towards a panel of tenofovir phosphonoamidate prodrugs. Incubation of both enzymes with 14C-labeled GS-7340 or [3H]difluorophosphonate resulted in the covalent labeling of identical 29-kDa catalytic subunits. Finally, following a 4-h incubation with GS-7340 and GS-9131, the intracellular concentrations of prodrug metabolites detected in CatA-negative fibroblasts were approximately 7.5- and 3-fold lower, respectively, than those detected in normal control fibroblasts. Collectively, these data demonstrate the key role of CatA in the intracellular activation of nucleotide phosphonoamidate prodrugs and open new possibilities for further improvement of this important class of antiviral prodrugs.

摘要

GS - 7340和GS - 9131(分别为9 - [(R) - 2 - [[(S) - [[(S) - 1 - (异丙氧基羰基)乙基]氨基]苯氧基膦酰基]甲氧基] - 丙基]腺嘌呤和9 - (R) - 4' - (R) - [[[(S) - 1 - [(乙氧基羰基)乙基]氨基]苯氧基膦酰基]甲氧基] - 2' - 氟 - 1' - 呋喃基腺嘌呤)分别是替诺福韦(9 - R - [(2 - 膦酰基甲氧基)丙基]腺嘌呤,简称TFV)和一种环核苷酸类似物GS - 9148(膦酰基甲氧基 - 2' - 氟 - 2',3' - 二脱氧脱氢腺苷)的新型烷基丙氨酰苯基酯前药。这两种前药对野生型和耐药型人类免疫缺陷病毒1型毒株均表现出强效抗逆转录病毒活性,且具有优异的体内药代动力学特性。在本研究中,负责GS - 7340和GS - 9131细胞内活化第一步的主要酶活性从人外周血单核细胞中分离出来,并被鉴定为溶酶体羧肽酶A(组织蛋白酶A [CatA];EC 3.4.16.5)。纯化的水解酶的生化特性(天然复合物和催化亚基的分子量分别为100 kDa和29 kDa;等电点 [pI] 为5.5)与CatA相符。重组CatA和分离出的前药水解酶对抑制剂的敏感性相同,对一组替诺福韦膦酰胺前药的底物偏好也相同。用14C标记的GS - 7340或[3H]二氟膦酸酯孵育这两种酶,均导致相同的29 kDa催化亚基发生共价标记。最后,用GS - 7340和GS - 9131孵育4小时后,在CatA阴性成纤维细胞中检测到的前药代谢物细胞内浓度分别比正常对照成纤维细胞中检测到的低约7.5倍和3倍。总体而言,这些数据证明了CatA在核苷酸膦酰胺前药细胞内活化中的关键作用,并为进一步改进这类重要的抗病毒前药开辟了新的可能性。

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