class="enumerated" style="list-style-type:decimal">Following an intracellular alkali load (imposed by acetate prepulsing in CO2/HCO3− buffer), intracellular pH (pHi) of the guinea-pig ventricular myocyte (recorded from intracellular SNARF fluorescence) recovers to control levels. Recovery has two phases. An initial rapid phase (lasting up to 2 min) is followed by a later slow phase (several minutes). Inhibition of sarcolemmal acid-loading carriers (by removal of extracellular Cl−) inhibits the later, slow phase but the initial rapid recovery phase persists. It also persists in the absence of extracellular Na+ and in the presence of the HCO3− transport inhibitor DIDS (4,4-di-isothiocyanatostilbene-2,2-disulphonic acid).The rapid recovery phase is not evident if the alkali load has been induced by reducing PCO2 (from 10 to 5 %), and it is inhibited in the absence of CO2/HCO3− buffer (i.e. Hepes buffer). It is also slowed by the carbonic anhydrase (CA) inhibitor acetazolamide (ATZ). We conclude that it is caused by buffering of the alkali load through the hydration of intracellular CO2 (CO2-dependent buffering).The time course of rapid recovery is consistent with an intracellular CO2 hydration rate constant (k1) of 0.36 s−1 in the presence of CA activity, and 0.14 s−1 in the absence of CA activity. This latter k1 value matches the literature value for uncatalysed CO2 hydration in free solution. Natural CO2 hydration is accelerated 2.6-fold in the ventricular myocyte by endogenous CA.The rapid recovery phase represents a period when the intracellular CO2/HCO3− buffer is out of equilibrium (OOE). Modelling of the recovery phase using our k1 value, indicates that OOE conditions will normally extend for at least 2 min following a step rise in pHi (at constant PCO2). If CA is inactive, this period can be as long as 5 min. During normal pHi regulation, the recovery rate during these periods cannot be used as a measure of sarcolemmal acid loading since it is a mixture of slow CO2-dependent buffering and transmembrane acid loading. The implication of this finding for quantification of pHi regulation during alkalosis is discussed.
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机译:class =“ enumerated” style =“ list-style-type:decimal”> <!-list-behavior =枚举前缀-word = mark-type = decimal max-label-size = 0-> 在细胞内碱负荷(由乙酸盐在CO2 / HCO3 -缓冲液中预脉冲施加)之后,豚鼠心室肌细胞的细胞内pH(pHi)(从细胞内SNARF荧光记录)恢复到控制水平。恢复分为两个阶段。最初的快速阶段(持续2分钟),随后是缓慢的阶段(几分钟)。抑制装载肌膜酸的载体(通过去除细胞外Cl -)抑制了后期的缓慢阶段,但最初的快速恢复阶段仍然存在。在没有细胞外Na + 和HCO3 -运输抑制剂DIDS(4,4-di-isothiocyanatostilbene-2,2-disulphonic acid)的情况下,它也持续存在。 )。 如果通过减少PCO2(从10%到5%)诱导了碱负荷,则快速恢复阶段并不明显,并且在没有CO2 / HCO3 -< / sup>缓冲区(即Hepes缓冲区)。碳酸酐酶(CA)抑制剂乙酰唑胺(ATZ)也会减慢其速度。我们得出结论,这是由于通过细胞内CO2的水合缓冲碱负荷(CO2依赖性缓冲液)引起的。 快速恢复的时间过程与细胞内CO2的水合速率常数(k1)一致在存在CA活动的情况下为0.36 s -1 ,而在没有CA活动的情况下为0.14 s -1 。后一个k1值与自由溶液中未催化的CO2水合的文献值匹配。内源性CA可使心室肌细胞的天然CO2水合加速2.6倍。 快速恢复阶段代表细胞内CO2 / HCO 3 - sup>缓冲区不平衡(OOE)。使用我们的k 1 值对恢复阶段进行建模,表明在pH i 逐步升高之后,OOE条件通常会持续至少2分钟(在恒定的P CO 2 )。如果CA处于非活动状态,则此期间可能长达5分钟。在正常的pH i 调节过程中,这些时间段的回收率不能用作肌膜酸负荷的量度,因为它是缓慢的CO 2 依赖型缓冲液和跨膜的混合物酸负荷。讨论了这一发现对定量碱中毒过程中pH i 调节的意义。
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