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大鼠器官和人血清中的氨肽酶P活性。

Aminopeptidase P activity in rat organs and human serum.

作者信息

Holtzman E J, Pillay G, Rosenthal T, Yaron A

出版信息

Anal Biochem. 1987 May 1;162(2):476-84. doi: 10.1016/0003-2697(87)90423-4.

Abstract

The substrate Lys(epsilon-Dnp)-Pro-Pro-NH-CH2-CH2-NH-ABz in which the fluorescent 2-aminobenzoyl (ABz) group (lambda ex = 320, lambda em = 410 nm) is intramolecularly quenched by the 2,4-dinitrophenyl (Dnp) chromophore was synthesized and used for the development of a sensitive assay for aminopeptidase P (EC 3.4.11.9). The emission of the intact compound was 160 times less than that of an equimolar concentration of Pro-Pro-NH-CH2-CH2-NH-ABz under the same conditions. The efficient resonance energy transfer permits an increased assay sensitivity as compared to the previously reported Phe(p-NO2)-Pro-Pro-NH-CH2-CH2-NH-ABz in which the p-nitrophenylalanyl [Phe(p-NO2)] residue caused only a 3.4-fold collisonal quenching. The kinetic constants Km were determined as 100 +/- 3.0 and 38 +/- 1.0 microM (mean of four experiments) for the human serum and the rat-lung enzymes, respectively. Both enzymes were inhibited by metal chelating agents and were not affected by 2.8 microM diisopropyl fluorophosphate. The mean activity in the sera of 53 healthy adults was 37.4 +/- 2.7 (standard error) with a standard deviation of 19.2 units/ml of serum. Only 10 microliters of serum was required for a reliable assay of the enzyme. The specific activity in rat-organ extracts was determined. High aminopeptidase P activity was observed in the testis, lung, kidney, and ovary and lower activity was observed in the serum.

摘要

合成了底物Lys(ε-Dnp)-Pro-Pro-NH-CH2-CH2-NH-ABz,其中荧光2-氨基苯甲酰基(ABz)基团(激发波长λex = 320,发射波长λem = 410 nm)被2,4-二硝基苯基(Dnp)发色团分子内淬灭,并将其用于开发一种灵敏的氨肽酶P(EC 3.4.11.9)检测方法。在相同条件下,完整化合物的发射强度比等摩尔浓度的Pro-Pro-NH-CH2-CH2-NH-ABz低160倍。与先前报道的Phe(p-NO2)-Pro-Pro-NH-CH2-CH2-NH-ABz相比,有效的共振能量转移提高了检测灵敏度,其中对硝基苯丙氨酰基[Phe(p-NO2)]残基仅引起3.4倍的碰撞淬灭。测定人血清和大鼠肺酶的动力学常数Km分别为100±3.0和38±1.0 μM(四个实验的平均值)。两种酶均受到金属螯合剂的抑制,且不受2.8 μM氟磷酸二异丙酯的影响。53名健康成年人血清中的平均活性为37.4±2.7(标准误),血清标准差为19.2单位/毫升。可靠检测该酶仅需10微升血清。测定了大鼠器官提取物中的比活性。在睾丸、肺、肾和卵巢中观察到高氨肽酶P活性,而在血清中观察到较低活性。

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