长白山白眉蝮蛇蛇毒精氨酸酯酶1的研究Ⅱ.酶学性质和荧光光谱研究(续I)

测得了长白山白眉蝮蛇毒精氨酸酯酶１的最适反应的ＰＨ范围为７．０－８．０,且与酶反应底物对甲苯磺酰－Ｌ－精氨酸甲酯的反应无明显的最适应反应温度,荧光光谱的研究结果表明：该酶的酪氨酸残基的荧光被色氨酸残基的荧光所掩盖;同步荧光光谱结果表明：当发射波长与激素波长差△λ分别为２０ｎｍ和７５ｎｍ时,精氨酸酯酶１的荧光光谱分别由酪氨酸和色氨酸残基所贡献,且处于亲水性环境中;精氨酸酯酶１的荧光发射强度受溶液酸度     

稀土及其配合物对蛇毒磷脂酶A_2活性的影响

分别研究了三价稀土离子 (La3 + ,Eu3 + ,Dy3 + ,Yb3 + )、二乙三胺五乙酸及其衍生物二乙三胺五乙酸 -双二甲酰胺 ,二乙三胺五乙酸 -双 (异烟肼 )与稀土离子的配合物以及Tb -谷氨酰胺配合物对蛇毒磷脂酶A2 活性的影响 .浓度低于 <3μmol/L的稀土离子可以激活磷脂酶A2 ,浓度大于 5 μmol/L后稀土离子对酶活性表现出抑制作用 ;外源Ca2 + 离子的加入可以缓解稀土离子对酶活性的抑制作用 ,表明稀土离子和钙离子是竞争性地结合在酶的活性部位 ;稀土离子和二乙三胺五乙酸及其衍生物的配合物对酶活性没有明显影响 ;Tb -谷氨酰胺在浓度大于 10 μmol/L后开始抑制酶的活性     

长白山白眉蝮蛇蛇毒精氨酸酯酶1的研究Ⅱ.酶学性质和荧光光谱研究(续Ⅰ)

测得了长白山白眉蝮蛇毒精氨酸酯酶 1的最适反应的pH范围为 7.0～ 8.0 ,且与酶反应底物对甲苯磺酰-L -精氨酸甲酯 (TAME)的反应无明显的最适应反应温度 .荧光光谱的研究结果表明 :该酶的酪氨酸残基的荧光被色氨酸残基的荧光所掩盖 ;同步荧光光谱结果表明 :当发射波长与激发波长差Δλ分别为 2 0nm和 75nm时 ,精氨酸酯酶 1的荧光光谱分别由酪氨酸 (Tyr)和色氨酸 (Trp)残基所贡献 ,且处于亲水性环境中 ;精氨酸酯酶 1的荧光发射强度受溶液酸度变化的影响 .I- ,Acr和NBS对精氨酸酯酶 1的荧光淬灭结果表明这种酶中含有多个色氨酸残基 ,且处于不同的微环境中。     

一种钙/钙调蛋白依赖性的蛇毒磷脂酶A2

稀土离子;活性;一种钙/钙调蛋白依赖性的蛇毒磷脂酶A2     

尖吻蝮蛇蛇毒出血毒素Ⅲ的荧光光谱

皖南尖吻蝮蛇蛇毒经分离和纯化得到出血毒素Ⅲ(AaH Ⅲ),质谱测定分子量为23,284.4±0.1。实验表明,Trp残基较大程度位于AaH Ⅲ分子的疏水区。十二烷基磺酸钠(SDS)和盐酸胍的加入使AaH Ⅲ的分子构象发生变化,导致分子内色氨酸(Trp)残基的荧光淬灭。盐酸胍的加入使Trp残基的荧光发射峰位明显红移,表明位于AaH Ⅲ分子较疏水环境的Trp残基相对外露。我们还就酸度、EDTA和金属离子对AaH Ⅲ分子内Trp残基荧光光谱的影响进行了研究和讨论。     

pBPB共价修饰蝮蛇酸性磷脂酶A2的晶体学数据

The Crystals of acidic phospholipase A2 from the venom of Agkistrodon blomhoffii brevicaudus (i.e. Agkistrodon halys pallas) covalently modified with p-bromo-phenacylbromide were obtained by the method of hanging drop vapor diffusion. Crystallization droplet was composed of 0.06mol?L-1 Na(CH3)2AsO2 (pH=6.5), 24.8% (v/v) 1,4-butanediol, and 4.5mg?mL-1 protein. The crystal data are of a=b=82.82?., c=32.85?, space group P61. 8945 unique reflections with 1.93 ? resolution were measured on a Siemens area detector X-ray diffractometor, of which 8069 reflections having F0 >2σ(F). The experimental results show that the crystals are suitable to a structure analysis of high resolution.     

长白山白眉蝮蛇蛇毒精氨酸酯酶1的研究Ⅰ.纯化、分子量测定及纯度鉴定

利用离子交换 (DEAESephadexA - 50 )和凝胶过滤层析 (SephadexG - 75)技术首次从长白山白眉蝮蛇蛇毒 (AgkistrodonblomhoffiiUssurensis)中纯化得到了一种精氨酸酯酶纯品。经SDS -聚丙烯酰胺凝胶电泳(SDS -PAGE)以及基质辅助激光解吸电离飞行时间质谱 (MALDI/TOF/MS)鉴定为单一纯蛋白 ,分子量为2 991 8.5± 1 5Da ,为进一步研究其结构与功能提供了可靠的依据。     

白眉蝮蛇蛇毒和蛇毒酶的基质辅助激光解吸电离飞行时间质谱法研究

应用基质辅激光解吸电离飞行时间质谱（ＭＡＬＤＩ－ＴＯＦ－ＭＳ）法对长白山眉蝮蛇蛇毒和纯化得到的两种蛇毒酶进行了研究,得到了它们的分子质量并验证了纯度。同时还考察了不同产地的蛇毒、蛇毒蛋白浓度以及基质对分析结果的影响,实验结果表明ＭＡＬＤＩ－ＴＯＦ－ＭＳ法是检测蛋白纯化过程和分析蛋白相对分子质量十分有效的手段。     

白眉蝮蛇蛇毒及蛇毒酶的激光解吸飞行时间质谱研究

Perkins等[1]用MALDI/TOF/MS对不同种类蛇毒中神经毒素进行了分析,彭嘉柔等[2,3]对江浙蝮蛇和蛇毒粗组份进行了初步质谱表征.但蛇毒蛋白纯化困难,因此对单一组份的研究较少且不系统.本文以白眉蝮蛇蛇毒(AgkistrodonblomhoffiiUssurensis,ABUV)为原料,纯化得到了精氨酸酯酶(Arginineesterase,AEase)、磷脂酶A2(PhospholipaseA2,PLA2)、纤溶酶(fibrinolyticenzyme)和L-氨基酸氧化酶(L-aminoacidoxidase),并且用MALDI/TOF/MS法对它们和蛇毒粗毒进行了系统研究.1　实验部分1.1　仪器和药品　激光解吸质谱仪为美国Molecular公司L…     

长白山白眉蝮蛇蛇毒酶的基质辅助激光解吸质谱分析

用基质辅助激光解吸飞行时间质谱法对长白山眉蝮蛇蛇毒所含４种主要酶：磷脂酶Ａ２,精氨酸酯酶,纤溶酶及Ｌ－氨基酸氧化酶进行了纯度鉴定和分子量测定,结果表明ＭＡＬＤＩ－ＴＯ－ＦＭＸ具有灵敏度高,分辨能力强,分析时间短及样品用量少等优点。用ＭＡＬＤＩ－ＴＯＦＭＳ法分析蛇毒酶的纯度和分子量简捷,快速且重现性好,是ＳＤＳ聚丙烯酰胺凝胶电泳所无法比拟的。     

一种钙/钙调蛋白依赖性的蛇毒磷脂酶A_2

分别研究了钙离子和三价稀土离子对白眉蝮蛇 (Agkistrodon blomhoffii Ussurensis)蛇毒磷脂酶 A2(PLA2 )活性的影响以及钙调蛋白对它的激活作用 .实验结果表明 ,PLA2 的活性对钙离子表现出依赖性 ,钙调蛋白能够激活该蛇毒 PLA2 ,钙调蛋白的拮抗剂三氟甲基吩噻嗪 (Trifluoperazine)能够完全抑制它对 PLA2的激活作用 .三价稀土离子 La3 、Eu3 、Dy3 、Yb3 对该 PLA2 的活性表现出抑制作用 ,其中离子半径较大的La3 和 Eu3 对酶活的抑制程度要小于半径较小的 Dy3 和 Yb3 .     

Phospholipase A2-Catalyzed Hydrolysis of 1,2-DimyristoyI-sn-Glycero-3-Phosphocholine in Organic Solvents

The phospholipase A2-catalyzed hydrolysis of phosphatidylcholine in organic solvents is described. The effects of various sources of enzymes are discussed; among five phospholipases A2, bee venom enzyme has the greatest activity, Naja naja venom and Naja mocambique enzymes have moderate activities, and pancreatic enzymes have the least activities. The effects of adducts such as alcohols, ether, and bovine serum albumin in chloroform on this catalysis are discussed; adducts, such as ether or alcohol, in small proportions increased the hydrolysis rate, but in large proportions inhibited hydrolysis. Bovine serum albumin increased slightly the phospholipase A2 catalysis rate. From the effect of temperature on this catalysis in chloroform, the substrate conformation at the α-memylcne region of acyl chains is a major factor for activation of phospholipases A2, confirming our previous conclusion that the substrate conformation is an important factor in the activation of phospholipase A2.     

正交晶型江浙蝮蛇毒碱性磷脂酶A2初步结晶学研究

The basic phospholipase A2 from the venom of Agkistrodon halys pallas possesses the ability to cause hemolysis in contrast to the other two phospholipase A2 from the same venom. A new form of crystals of this enzyme was grown. The crystals belong to space group of P212121 with unit cell parameters of a=9.175nm, b=10.080nm , c=2.287nm.The crystals diffract to high resolution, and are suitable for detailed structural studies. The data were collected up to 0.25nm resolution using synchrotron radiation-imaging plate-Weissenberg camera system. Preliminary analysis reveals the presence of two molecules in the asymmetric uint and the molecule may pack with the smallest dimension approximately parallel to the c axis. The new crystal form is more attractive than the monoclinic one previously reported for crystallographic structure determination as it contains fewer molecules in the asymmetric unit.     

Synthesis of Competitive Inhibitors of Phospholipase A 2 (PLA 2 )

The synthetic routes for preparation of several phospholipid analogues such as lithium alkyl-3-alkoxy allylvinyl-sn-glycerol 5 and 6 and lithium trans-2-amidomethyl phosphate 7 and lithium cholesterol ester phosphate 8 containing ether, amide, and phosphate ester moieties are described.