碳酸酐酶的同工酶：动力学特性，特别涉及在肠道中的功能。

The isoenzymes of carbonic anhydrase: kinetic properties with particular reference to the functions in the intestinal tract.

作者信息

Carter M J, Parsons D S

出版信息

J Physiol. 1972 Jan;220(2):465-78. doi: 10.1113/jphysiol.1972.sp009716.

DOI:10.1113/jphysiol.1972.sp009716

PMID:4622484

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1331712/

Abstract

Details are given of an electrometric method for measuring the activity of isoenzymes of carbonic anhydrase (EC 4.2.1.1) in catalysing the hydration of carbon dioxide under different conditions at 0 degrees C. In the method, a measured volume of water saturated with carbon dioxide at a known partial pressure and appropriate temperature is introduced into a buffered solution. Using a sensitive electrometer and recording instrument, the subsequent change in hydrogen ion concentration is recorded as a function of time. Under the conditions of assay, the pH change induced in the presence of substrate is very small (DeltapH < 0.05 units) and the period of observation need not exceed 10 sec.2. For enzymes isolated from guinea-pig tissues, it is found that the specific activity of the ;high activity' isoenzyme (carbonic anhydrase C, carbonic anhydrase II, HACA) is about eighteen times that of the ;low activity' counterpart (carbonic anhydrase B, carbonic anhydrase I, LACA) when measured at 0 degrees C, pH 7.2, and ionic strength 0.19. Under the same conditions, the K(m) was found to be 10 mM for the ;high activity' isoenzyme and 23 mM for the ;low activity' isoenzyme. No differences were found between the equivalent kinetic parameters of the corresponding isoenzymes isolated from different tissues.3. The isoenzymes isolated from guinea-pig tissues are found to be inhibited by acetazolamide in a non-competitive manner. It is also found that the ;high activity' isoenzyme is many times more sensitive to this inhibitor than is the ;low activity' isoenzyme. Evidence is presented which indicates that one acetazolamide binding site is present on each molecule of either isoenzyme.4. While chloride ions specifically inhibit the ;low activity' component of guinea-pig carbonic anhydrase (I(0.5) = 40 mM), acetate, butyrate and pyruvate inhibit both isoenzymes. Under the conditions employed, acetate and pyruvate are more strongly inhibitory to the ;low activity' isoenzyme than to the ;high activity' isoenzyme, while butyrate is more strongly inhibitory to the ;high activity' isoenzyme.5. The findings are discussed with particular reference to the physiological significance of the presence of the isoenzymes in the gastro-intestinal tract. Also considered are possible relationships between the distribution of the ;low activity' isoenzyme in these tissues and the transport and metabolism of products of fermentation occurring in the intestinal lumen.

摘要

本文详细介绍了一种通过测量在0℃不同条件下碳酸酐酶（EC 4.2.1.1）同工酶催化二氧化碳水合反应的活性的电位测定法。该方法是将在已知分压和适当温度下用二氧化碳饱和的一定体积的水引入缓冲溶液中。使用灵敏的静电计和记录仪器，记录氢离子浓度随时间的变化。在测定条件下，底物存在时引起的pH变化非常小（ΔpH＜0.05单位），观察时间无需超过10秒。
对于从豚鼠组织中分离得到的酶，发现在0℃、pH 7.2和离子强度0.19条件下测定时，“高活性”同工酶（碳酸酐酶C、碳酸酐酶II、HACA）的比活性约为“低活性”对应物（碳酸酐酶B、碳酸酐酶I、LACA）的18倍。在相同条件下，“高活性”同工酶的米氏常数（K(m)）为10 mM，“低活性”同工酶为23 mM。从不同组织分离得到的相应同工酶的等效动力学参数之间未发现差异。
发现从豚鼠组织中分离得到的同工酶受到乙酰唑胺的非竞争性抑制。还发现“高活性”同工酶对该抑制剂的敏感性比“低活性”同工酶高许多倍。有证据表明，每种同工酶的每个分子上都存在一个乙酰唑胺结合位点。
虽然氯离子特异性抑制豚鼠碳酸酐酶的“低活性”组分（I(0.5)=40 mM），但乙酸盐、丁酸盐和丙酮酸盐抑制两种同工酶。在所采用的条件下，乙酸盐和丙酮酸盐对“低活性”同工酶的抑制作用比对“高活性”同工酶更强，而丁酸盐对“高活性”同工酶的抑制作用更强。
结合胃肠道中同工酶存在的生理意义对这些发现进行了讨论。还考虑了这些组织中‘低活性’同工酶的分布与肠腔中发酵产物的转运和代谢之间可能的关系。