Garcia J G, Siflinger-Birnboim A, Bizios R, Del Vecchio P J, Fenton J W, Malik A B
J Cell Physiol. 1986 Jul;128(1):96-104. doi: 10.1002/jcp.1041280115.
We studied the effect of thrombin on albumin permeability across the endothelial monolayer in vitro. Bovine pulmonary artery endothelial cells were grown on micropore membranes. Morphologic analysis confirmed the presence of a confluent monolayer with interendothelial junctions. Albumin permeability was measured by the clearance of 125I-albumin across the endothelial monolayer. The control 125I-albumin clearance was 0.273 +/- 0.02 microliter/min. The native enzyme, alpha-thrombin (10(-6) to 10(-10) M), added to the luminal side of the endothelium produced concentration-dependent increases in albumin clearance (maximum clearance of 0.586 +/- 0.08 microliter/min at 10(-6) M). Gamma (gamma) thrombin (10(-6) M and 10(-8) M), which lacks the fibrinogen recognition site, also produced a concentration-dependent increase in albumin clearance similar to that observed with alpha-thrombin. Moreover, the two proteolytically inactive forms of the native enzyme, i-Pr2 P-alpha-thrombin and D-Phe-Pro-Arg-CH2-alpha-thrombin, increased the 125I-albumin clearance (0.610 +/- 0.09 microliter/min and 0.609 +/- 0.02 microliter/min for i-Pr2 P-alpha-thrombin and D-Phe-Pro-Arg-CH2-alpha-thrombin at 10(-6) M, respectively). Since the modified forms of thrombin lack the fibrinogen recognition and active serine protease sites, the results indicate that neither site is required for increased albumin permeability. The increase in albumin clearance with alpha-thrombin was not secondary to endothelial cell lysis because lactate dehydrogenase concentration in the medium following thrombin was not significantly different from baseline values. There was also no morphological evidence of cell lysis. Moreover, the increase in 125I-albumin clearance induced by alpha-thrombin was reversible by washing thrombin from the endothelium. The basis for the increased albumin permeability following the addition of alpha-thrombin appears to be a reversible change in endothelial cell shape with formation of intercellular gaps.
我们在体外研究了凝血酶对白蛋白透过内皮单层的影响。牛肺动脉内皮细胞生长在微孔膜上。形态学分析证实存在具有内皮间连接的融合单层。通过125I-白蛋白透过内皮单层的清除率来测量白蛋白通透性。对照125I-白蛋白清除率为0.273±0.02微升/分钟。添加到内皮管腔侧的天然酶α-凝血酶(10^(-6)至10^(-10) M)使白蛋白清除率呈浓度依赖性增加(在10^(-6) M时最大清除率为0.586±0.08微升/分钟)。缺乏纤维蛋白原识别位点的γ(γ)凝血酶(10^(-6) M和10^(-8) M)也使白蛋白清除率呈浓度依赖性增加,类似于α-凝血酶所观察到的情况。此外,天然酶的两种无蛋白水解活性形式,异丙基-2-脯氨酸-α-凝血酶和D-苯丙氨酸-脯氨酸-精氨酸-CH2-α-凝血酶,增加了125I-白蛋白清除率(在10^(-6) M时,异丙基-2-脯氨酸-α-凝血酶和D-苯丙氨酸-脯氨酸-精氨酸-CH2-α-凝血酶的清除率分别为0.610±0.09微升/分钟和0.609±0.02微升/分钟)。由于凝血酶的修饰形式缺乏纤维蛋白原识别和活性丝氨酸蛋白酶位点,结果表明增加白蛋白通透性两者位点均非必需。α-凝血酶引起的白蛋白清除率增加并非内皮细胞裂解的继发结果,因为凝血酶作用后培养基中乳酸脱氢酶浓度与基线值无显著差异。也没有细胞裂解的形态学证据。此外,通过从内皮中洗去凝血酶,α-凝血酶诱导的125I-白蛋白清除率增加是可逆的。添加α-凝血酶后白蛋白通透性增加的基础似乎是内皮细胞形状的可逆变化以及细胞间隙的形成。
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