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A single-cell technique for the measurement of membrane potential membrane conductance and the efflux of rapidly penetrating solutes in Amphiuma erythrocytes

机译:单细胞技术用于测量两栖红细胞中膜电位膜电导和快速渗透的溶质的流出

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摘要

We describe a single-cell technique for measuring membrane potential, membrane resistance, and the efflux of rapidly penetrating solutes such as Cl and H2O. Erythrocytes from Amphiuma means were aspirated into a Sylgard (Dow Corning Corp.)-coated capillary. The aspirated cell separated a solution within the capillary from a solution in the bath. Each of these two solutions was contiguous with approximately 5% of the total membrane surface. Microelectrodes placed concentrically within the capillary permit the measurement of intracellular voltage, specific membrane resistance, and the electrical seal between the two solutions. The intracellular voltage averaged -17.7 mV (pH 7.6) and changed as either intra- or extracellular chloride was varied. The average specific membrane resistance measured by passing current across the exposed membrane surface was 110 ohm-cm2. 36Cl and tritiated H2O fluxes (0.84 +/- 0.05 x 10(-6) M . cm-2 . min-1 and 6.4 +/- 1.5 x 10(-3) M . cm-2 . min-1, respectively) were determined by noting the rate at which isotope leaves the cell and crosses the membrane exposed to the bath. Our measured values for the flux of 36Cl and tritiated H2O approximate reported values for free-floating cells. 36Cl efflux, in addition, is inhibited by 4-acetamido-4'-isothiocyano-stilbene 2,2'-disulfonic acid (SITS) and furosemide, known inhibitors of the anion exchange mechanism responsible for the rapid anion fluxes of red blood cells. One can also demonstrate directly that > 89% of 36Cl efflux is "electrically silent" by analyzing the flux in the presence of an imposed transcellular voltage.
机译:我们描述了一种单细胞技术,用于测量膜电势,膜电阻以及快速渗透的溶质(例如Cl和H2O)的流出。将来自Amphiuma装置的红细胞吸到Sylgard(Dow Corning Corp.)涂层的毛细管中。抽吸池将毛细管内的溶液与浴中的溶液分离。这两种溶液中的每一种都是连续的,约占总膜表面的5%。同心放置在毛细管内的微电极可以测量细胞内电压,比膜电阻和两种溶液之间的电密封。细胞内电压平均为-17.7 mV(pH 7.6),并且随着细胞内或细胞外氯化物的变化而变化。通过使电流流过暴露的膜表面而测得的平均比膜电阻为110 ohm-cm2。 36Cl和tri化的H2O通量(分别为0.84 +/- 0.05 x 10(-6)M.cm-2.min-1和6.4 +/- 1.5 x 10(-3)M.cm-2.min-1)通过记录同位素离开细胞并穿过暴露于镀液中的膜的速率来确定离子强度。我们测得的36Cl和H化H2O通量的测量值近似于自由漂浮电池的报告值。此外,36Cl外排还受4-乙酰氨基-4'-异硫氰基-二苯乙烯2,2'-二磺酸(SITS)和呋塞米的抑制,呋塞米是引起红细胞快速阴离子通量的阴离子交换机制抑制剂。一个人还可以通过在施加跨细胞电压的情况下分析通量来直接证明> 89%的36Cl外排是“电沉默的”。

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