Chen H, Namkung M J, Juchau M R
Department of Pharmacology, School of Medicine, University of Washington, Seattle 98195, USA.
Biochem Pharmacol. 1995 Oct 12;50(8):1257-64. doi: 10.1016/0006-2952(95)02005-w.
Catalysis of the oxidation of all-trans-retinol (vitamin A1) or of all-trans-retinal to all-trans-retinoic acid (all-trans-RA) by rat conceptal enzymes was investigated during organogenesis. Products of the reaction were identified and quantified with HPLC by comparing their elution times with those of authentic standard retinoids. Under the incubation and assay conditions utilized, all-trans-retinol and all-trans-retinal were converted to readily detectable quantities of all-trans-RA. Rat conceptal homogenates from gestational days 10.5, 11.5 and 12.5 each exhibited enzymatic activity for oxidation of all-trans-retinol and all-trans-retinal to all-trans-RA. Enzymatic catalysis was verified by showing that: (1) both reactions were coenzyme dependent; (2) the rates of reactions increased as concentrations of conceptal protein increased; (3) both reactions were abolished by heating the tissue homogenates (100 degrees, 5 min); and (4) both reactions exhibited substrate saturation. Under the same experimental conditions, formation of all-trans-RA from all-trans-retinol was much slower than from all-trans-retinal, suggesting that oxidation of all-trans-retinol to all-trans-retinal was the rate-limiting step for biotransformation of all-trans-retinol to all-trans-RA in embryonic tissues. When NAD or NADP were replaced by NADH or NADPH, the rate of oxidation of all-trans-retinol was reduced markedly, indicating that the reaction was catalyzed primarily by an NAD/NADP-dependent dehydrogenase(s). Carbon monoxide (CO:O2 = 90:10) did not inhibit the reaction. NAD appeared to be a more effective cofactor than NADP in catalyzing oxidation of all-trans-retinal to all-trans-RA. When NAD was omitted, formation of all-trans-RA from all-trans-retinal was reduced by approximately 55%. Replacing NAD by NADH or NADPH also reduced the conversion of all-trans-retinal to all-trans-RA by about 60%. These observations suggested at least two pathways for the generation of all-trans-RA from all-trans-retinal in embryos: oxidation catalyzed by an NAD/NADP-dependent dehydrogenase(s) and oxidation catalyzed by an oxidase(s) that did not require NAD, NADH, NADP or NADPH. Conversion of all-trans-retinol to all-trans-RA was inhibited strongly by low concentrations of citral, but not by high concentrations of sodium azide, 4-methylpyrazole, or metyrapone. Similarly, oxidation of all-trans-retinal was inhibited strongly by citral but not by metyrapone.(ABSTRACT TRUNCATED AT 400 WORDS)
在器官发生过程中,研究了大鼠胚胎酶对全反式视黄醇(维生素A1)或全反式视黄醛氧化为全反式视黄酸(全反式RA)的催化作用。通过将反应产物的洗脱时间与标准视黄类化合物的洗脱时间进行比较,用高效液相色谱法对反应产物进行鉴定和定量。在所采用的孵育和测定条件下,全反式视黄醇和全反式视黄醛被转化为易于检测到的全反式RA。来自妊娠第10.5、11.5和12.5天的大鼠胚胎匀浆均表现出将全反式视黄醇和全反式视黄醛氧化为全反式RA的酶活性。通过以下几点验证了酶催化作用:(1)两个反应均依赖辅酶;(2)反应速率随胚胎蛋白浓度的增加而增加;(3)加热组织匀浆(100摄氏度,5分钟)可使两个反应均被消除;(4)两个反应均表现出底物饱和。在相同的实验条件下,全反式视黄醇生成全反式RA的速度比全反式视黄醛慢得多,这表明全反式视黄醇氧化为全反式视黄醛是胚胎组织中全反式视黄醇生物转化为全反式RA的限速步骤。当用NADH或NADPH替代NAD或NADP时,全反式视黄醇的氧化速率显著降低,表明该反应主要由NAD/NADP依赖性脱氢酶催化。一氧化碳(CO:O2 = 90:10)不抑制该反应。在催化全反式视黄醛氧化为全反式RA方面,NAD似乎比NADP更有效。当省略NAD时,全反式视黄醛生成全反式RA的量减少约55%。用NADH或NADPH替代NAD也使全反式视黄醛向全反式RA的转化降低约60%。这些观察结果表明,胚胎中全反式视黄醛生成全反式RA至少有两条途径:由NAD/NADP依赖性脱氢酶催化的氧化作用和由不需要NAD、NADH、NADP或NADPH的氧化酶催化的氧化作用。低浓度的柠檬醛强烈抑制全反式视黄醇向全反式RA的转化,但高浓度的叠氮化钠、4-甲基吡唑或甲吡酮则无此作用。同样,柠檬醛强烈抑制全反式视黄醛的氧化,但甲吡酮则无此作用。(摘要截短于400字)
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