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犬血清中骨碱性磷酸酶同工酶活性的定量分析。

Quantitation of skeletal alkaline phosphatase isoenzyme activity in canine serum.

作者信息

Farley J R, Hall S L, Ritchie C, Herring S, Orcutt C, Miller B E

机构信息

Department of Medicine, Loma Linda University, California.

出版信息

J Bone Miner Res. 1992 Jul;7(7):779-92. doi: 10.1002/jbmr.5650070708.

Abstract

Pursuing the hypothesis that quantitation of skeletal alkaline phosphatase (ALP) activity in canine serum would provide an index of the rate of bone formation, we compared three methods for isoenzyme-specific identification of skeletal ALP activity in canine serum: heat inactivation, wheat germ agglutinin (WGA) precipitation, and concanavalin A (ConA) precipitation. ALP isoenzyme activities were extracted from canine bone, intestine, and liver, diluted into heat-inactivated canine serum (i.e., serum without ALP activity), and used as calibrators of ALP isoenzyme activities. Differential sensitivity to inhibition by 10 mM L-homoarginine was used to distinguish intestinal ALP activity from hepatic and skeletal ALP activities (i.e., 9, 80, and 72% inhibition, respectively). To allow resolution of skeletal ALP activity from hepatic ALP activity, we tested two established methods (heat inactivation and WGA precipitation) and a novel method, ConA precipitation. The organ-derived skeletal and hepatic ALP isoenzyme activities were used to compare these three methods with respect to linearity, isoenzyme separation, and precision. All three methods were linear, but the WGA and ConA methods afforded greater isoenzyme separation and precision. The relative extent of isoenzyme separation (i.e., the difference in percentage remaining skeletal and hepatic ALP isoenzyme activities) averaged 23, 40, and 47% remaining ALP activity for the heat, WGA, and ConA methods, respectively. However, when these methods were applied to the quantitation of skeletal ALP activity in sera from 10 young and 10 adult beagles, the WGA method was found to be unacceptable because most of the results fell outside the range of the WGA assay calibrators (i.e., greater than 100% skeletal ALP activity). The heat and ConA methods showed that the amount of skeletal ALP activity in the beagle sera decreased with age, both as ALP activity per liter and as percentage of total serum ALP activity (p less than 0.001 for each). Skeletal ALP activity levels determined by ConA were correlated with values determined by heat inactivation (r = 0.87, p less than 0.001) but not with WGA-determined levels (r = 0.26). Intestinal ALP activity was detected in only 1 of these 20 sera. We conclude that ConA precipitation can be used for quantitation of skeletal ALP activity in beagle serum.

摘要

基于犬血清中骨骼碱性磷酸酶(ALP)活性定量可提供骨形成速率指标这一假设,我们比较了三种用于特异性鉴定犬血清中骨骼ALP活性的同工酶方法:热失活法、麦胚凝集素(WGA)沉淀法和刀豆球蛋白A(ConA)沉淀法。从犬的骨骼、肠道和肝脏中提取ALP同工酶活性,将其稀释到热失活的犬血清中(即无ALP活性的血清),用作ALP同工酶活性的校准物。利用10 mM L-高精氨酸抑制作用的差异敏感性来区分肠道ALP活性与肝脏和骨骼ALP活性(即分别抑制9%、80%和72%)。为了从肝脏ALP活性中分辨出骨骼ALP活性,我们测试了两种既定方法(热失活法和WGA沉淀法)以及一种新方法ConA沉淀法。使用器官来源的骨骼和肝脏ALP同工酶活性,从线性度、同工酶分离和精密度方面比较这三种方法。所有三种方法均呈线性,但WGA法和ConA法能实现更好的同工酶分离和精密度。热失活法、WGA法和ConA法的同工酶分离相对程度(即剩余骨骼和肝脏ALP同工酶活性百分比的差异)平均分别为剩余ALP活性的23%、40%和47%。然而,当将这些方法应用于10只幼犬和10只成年比格犬血清中骨骼ALP活性的定量时,发现WGA法不可接受,因为大多数结果超出了WGA检测校准物的范围(即骨骼ALP活性大于100%)。热失活法和ConA法表明,比格犬血清中骨骼ALP活性的量随年龄增长而降低,无论是以每升ALP活性还是以总血清ALP活性的百分比来衡量(每种情况p均小于0.001)。通过ConA法测定的骨骼ALP活性水平与通过热失活法测定的值相关(r = 0.87,p小于0.001),但与通过WGA法测定的水平不相关(r = 0.26)。在这20份血清中仅检测到1份含有肠道ALP活性。我们得出结论,ConA沉淀法可用于比格犬血清中骨骼ALP活性的定量。

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