首页> 美国卫生研究院文献>Canadian Journal of Comparative Medicine >Comparative effects of the human protein C activator Protac on the activated partial thromboplastin clotting times of plasmas with special reference to the dog.
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Comparative effects of the human protein C activator Protac on the activated partial thromboplastin clotting times of plasmas with special reference to the dog.

机译:人类蛋白C活化剂Protac对血浆中活化的部分凝血活酶凝结时间的比较作用特别是对狗的影响。

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摘要

The commercial snake venom extract, Protac, is a specific activator of the anticoagulant zymogen, protein C (PC) in human plasma. This specific action has led to its use in developing coagulation-based and amidolytic-based assays for the diagnosis of quantitative and/or qualitative PC deficiency states in human beings. The purpose of the present study was to compare the effects of Protac on the activated partial thromboplastin times (APTT) of human, bovine, equine, and canine plasmas in order to determine the potential value of this venom extract as an activator in functional PC assays in these domestic animal species. As expected, Protac significantly prolonged the APTT of normal human plasma, but had no effect on plasma known to be devoid of PC. Clotting times were prolonged by 34%-214% with concentrations of venom activator ranging from 0.1-1.0 U/mL. Under identical conditions, Protac prolonged the APTT of equine plasma by 11%-98% over control times. Even more dramatic was the inhibitory effect of Protac on the clotting of bovine plasma, extending the APTT more than 3-fold at a venom concentration of 0.1 U/mL. At higher venom concentrations, most bovine plasmas remained unclotted after 300 s (control time 34.1 s). Under similar conditions, the canine APTT was unaffected by Protac, even when the venom concentration was increased to 3 U/mL. In order to determine the reason for the lack in response of canine plasma, the concentration of the APTT reagent was altered (decreased), exposure time of the plasma to the Protac was increased from 2 min to 9 min, and the plasma was diluted to assess for the potential existence of plasma PC inhibitors. Protac caused an unexpected shortening of the APTT when the contact activator reagent was diluted. Increasing the exposure time had no effect. Although a slight prolongation of the canine APTT was detected when the plasma was diluted, the presence of strong plasma PC inhibition was considered an unlikely cause of the lack of significant anticoagulant action. The failure of Protac to exert a strong inhibitory effect on the canine APTT, as well as to generate amidolytic activity, suggests that this venom extract does not stimulate the production of activated PC activity in canine plasma. This may result from molecular differences in the canine PC molecule that prevent the formation of the stoichiometric complex of venom extract, APTT reagent, and canine protein, a complex thought to be essential for the PC-activating function of Protac. Protac may be suitable as an activator of PC in bovine and equine plasmas; however, it appears ineffective in generating anticoagulant activity in canine plasma.
机译:商业蛇毒提取物Protac是人血浆中抗凝酶原蛋白C(PC)的特定活化剂。该特定作用导致其在开发基于凝结和基于酰胺分解的测定中用于诊断人类中定量和/或定性PC缺乏状态。本研究的目的是比较Protac对人,牛,马和犬血浆血浆中活化的部分凝血活酶时间(APTT)的影响,以确定该蛇毒提取物在功能性PC分析中作为激活剂的潜在价值。在这些家畜物种中。如预期的那样,Protac显着延长了正常人血浆的APTT,但对已知不含PC的血浆没有影响。毒液激活剂的浓度范围为0.1-1.0 U / mL,凝血时间延长了34%-214%。在相同的条件下,Protac在控制时间内将马血浆的APTT延长了11%-98%。 Protac对牛血浆凝结的抑制作用更为显着,在毒液浓度为0.1 U / mL时,APTT扩展了3倍以上。在较高的毒液浓度下,大多数牛血浆在300 s(控制时间34.1 s)后仍未凝结。在类似条件下,即使毒液浓度增加到3 U / mL,犬APTT也不受到Protac的影响。为了确定犬血浆缺乏响应的原因,改变(降低)了APTT试剂的浓度,血浆对Protac的暴露时间从2分钟增加到9分钟,并将血浆稀释至评估血浆PC抑制剂的潜在存在。稀释接触活化剂后,Protac会导致APTT意外缩短。增加曝光时间没有影响。尽管在稀释血浆时检测到犬APTT略有延长,但血浆PC抑制作用强烈被认为是缺乏显着抗凝作用的不太可能的原因。 Protac不能对犬APTT产生强烈的抑制作用,并且不能产生酰胺分解活性,这表明这种毒液提取物不会刺激犬血浆中活化PC活性的产生。这可能是由于犬PC分子中的分子差异所致,该分子差异阻止了毒液提取物,APTT试剂和犬蛋白的化学计量复合物的形成,而这种复合物被认为对Protac的PC激活功能至关重要。 Protac可能适合作为牛和马血浆中PC的活化剂;然而,在犬血浆中产生抗凝活性似乎无效。

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