柞蚕卵组织蛋白酶B纯化及性质

昆虫卵内蛋白酶在胚胎发育中水解卵黄蛋白,为胚胎发育提供氨基酸。昆虫中已报道过几类卵蛋白酶,如家蚕中半胱氨酸蛋白酶和丝氨酸蛋白等。但是,目前尚不清楚这些蛋白酶是否存在于其他鳞翅目昆虫。了解这些蛋白酶的作用机理可以为我们提供害虫防治的新方法,并且,由于蛋白水解在许多生理过程中具有重要作用。如蛋白质的成熟和转运、受精、萌芽、肿瘤转移和其他形态发生等。因此,阐明这些蛋白酶的生物功能具有重要意义。由于Oi蚕卵粒大,产卵量也很大,因此被选作研究鳞翅目昆虫卵蛋白酶的材料,我们希望通过对数种昆虫卵内蛋白酶的研究,找出卵黄蛋白水解的一般规律。在我们前一篇文章中报道了oi蚕组织蛋白酶B的鉴定。该蛋白酶属于半胱酸蛋白酶类的组织蛋白,最适pH为3．5,可被E－64抑制。本文报道蛋白酶的纯化和蛋白质。经过5步纯化过程,从oi蚕卵母细胞中纯化出组织蛋白酶B,用SDS聚丙烯酰胺凝胶电泳测得蛋白酶的亚基分子量在47kDa左右。纯化的蛋白酶活性可被E－64和Leupeptin抑制。因此,该蛋白酶属于半胱氨酸蛋白酶。天冬氨酸蛋白酶特异性抑制Pepstatin不抑制其活性。其活性可被DFP和PMSF部分抑制制。这两种抑制剂通常抑制丝氨酸蛋白酶活性,但在家蚕中有报道,半氨酸蛋白也可被这两种抑制剂抑制。推测该知性中心除含有半胱氨酸残基外,可能还含有丝氨酸残基。由牛血红蛋白测得蛋白酶的最适pH为3．5。在pH3．5条件下对胚胎发育中蛋白酶活性变化进行了研究,并用纯化的蛋白酶制备了抗血清,采用单向免疫扩散对胚胎发育中组织蛋白酶B的含量进行了测定,结果表明这种蛋白酶在胚胎发育中含量较高,是胚肥发育中蛋白酶活性来源之一。     

昆虫卵内蛋白酶的研究

1　引言卵内蛋白酶在胚胎发育中水解卵黄蛋白 ,为胚胎发育提供氨基酸 ,如果卵内蛋白酶活性受到抑制 ,胚胎发育必然因为缺乏氨基酸而受阻 ,由此可见其对胚胎发育有重要意义。国外从 60年代开始以蝗虫为材料对昆虫卵内蛋白酶进行研究 (Kuk-Meiri,1 966) [1] ,但与卵黄蛋白相比 ,对昆虫卵内蛋白酶的研究少得多。到 80年代后期工作才逐渐多起来。先后被研究过的昆虫达 1 0余种 ,分属鳞翅目、双翅目、直翅目、蜚蠊目。迄今为止 ,已对蝗虫、家蚕、美洲大蠊、蜱等数种昆虫卵内蛋白酶进行了研究 ,其中以家蚕为材料做的工作最多。2　卵内蛋白酶的分…     

家蚕卵半胱氨酸蛋白酶纯化及抗血清制备

据报道,家蚕卵中存在半胱氨酸蛋白酶(Cysteine proteinase,CP),其性质与哺乳类溶酶体半胱氨酸蛋白酶类的组织蛋白酶L相似,最佳作用pH为3.5,体外最适作用底物为牛血红蛋白,体内最适作用底物为卵黄磷蛋白。经SDS—PAGE分析,分子量47KD。其主要作用是在胚胎发育过程中降解卵黄蛋白质,供胚胎发育之需要。 在成熟卵中具很高含量的半胱氨酸蛋白酶,在胚胎发育开始前,并不发生卵黄蛋白质的水解,其作用机制尚待阐明。为了进一步研究半胱氨酸蛋白酶的组织分布、合成位点、及cDNA克隆等,作者从家蚕卵中纯化了半胱氨酸蛋白酶,并制备了抗血清。     

棉铃虫卵内蛋白酶性质研究

在棉铃虫Helicoverpa armigera卵母细胞内检测到蛋白酶活性,其作用Ph在酸性范围,酶活性受E-64、Pepstatin和iPr₂P-F等多种抑制剂抑制。在Ph4.0时蛋白酶对牛血红蛋白有较高水解率。抗蓖麻蚕Philosamia cynthia ricini卵半胱氨酸蛋白酶血清和抗蓖麻蚕卵天冬氨酸蛋白酶血清可以识别棉铃虫卵内成分。实验结果表明;棉铃虫卵内可能存在半胱氨酸蛋白酶类、丝氨酸蛋白酶类和天冬氨酸蛋白酶类,并且与蓖麻蚕卵内蛋白酶有一定的相似性。     

蟾蜍细胞溶素的纯化及其生化特性研究

利用阴离子交换和凝胶过滤柱层析等方法对蟾蜍卵黄外被细胞溶素进行了分离纯化,获得了高纯度的样品．该酶的质量为３２ｋＤ,其特异性ＭＣＡ－人工合成底物为Ｂｏｃ－Ｇｌｎ－Ａｒｇ－Ａｒｇ－ＭＣＡ,能被ＤＦＰ、ＳＢＴＩ、ｌｅｕｐｅｐｔｉｎ和ｐ－ＡＭＰＳＦ等蛋白酶抑制剂所强烈抑制,但不受ｃｈｙｍｏｓｔａｔｉｎ、ｂｅｓｔａｔｉｎ、Ｅ－６４和ＥＤＴＡ等的影响,表明该酶是一种丝氨酸类型的蛋白酶     

慈菇蛋白酶抑制剂研究进展

蛋白酶抑制剂是一类能够抑制蛋白水解酶活性的物质。根据它们抑制的蛋白酶类型可分为丝氨酸、半胱氨酸、天冬氨酸、和金属蛋白酶抑制剂[1] 。由于它们能抑制昆虫肠道内以及一些病原微生物体内的蛋白酶[2～ 6 ] ,因此蛋白酶抑制剂在植物对昆虫和病原体的侵染防御系统中具有重要的作用。慈菇蛋白酶抑制剂Ａ、Ｂ是从慈菇球茎中分离纯化的双头多功能蛋白酶抑制剂 ,除了具备其他蛋白酶抑制剂在抗虫抗病方面的特点外 ,还有很多独特的优点。如 ,含量丰富、比活力高而且稳定 ;广谱性强 ;对胰蛋白酶、胰凝乳蛋白酶、激肽释放酶等多种蛋白酶有较强的抑…     

棉铃虫组织蛋白酶B组织分布与合成部位的研究

蛋白酶是指裂解肽链的所有酶类 ,根据作用位点的催化基团将蛋白酶分为 4大类 ,即丝氨酸蛋白酶、半胱氨酸蛋白酶 (ＣｙｓｔｅｉｎｅＰｒｏｔｅｉｎａｓｅｓ ,ＣＰ)、天冬氨酸蛋白酶和金属蛋白酶。每一大类又包括多种不同的蛋白酶 ,其中半胱氨酸蛋白酶是一类细胞内蛋白酶 ,包括组织蛋白酶Ｂ、Ｌ、Ｈ、Ｎ、Ｓ、Ｔ等 ,其活性中心含有活性必需的半胱氨酸残基 ,细胞内高度的还原环境对它们的作用非常重要 (Ｔｕｒｋ＆Ｂｏｂｔ,1991)。蛋白酶参与多种生理、病理性蛋白水解 ,在昆虫中的分布和功能也有报道 ,如蚊子卵中含有组织蛋白酶Ｂ ,参与胚胎发…     

蚯蚓体内一种纤溶酶原激活剂(e-PA)的部分性质研究

从赤子爱胜蚓（Ｅｉｓｅｎｉａｆａｅｔｉｄａ）中纯化出的一种纤溶酶原激活剂（ｅ－ＰＡ）在纤维蛋白平板上可表现出三种活性,分别记为：ＣＦＰｇ,ｕＣＦＰｇ和ｕＣＦ．为更好了解各种活性与ｅ－ＰＡ的纤溶能力的关系,考察了在ＳＤＳ和不同抑制剂存在下各种活性的变化．结果表明,ＳＤＳ可以增强ＣＦＰｇ活性且使得ｅ－ＰＡ变得对一些抑制剂更敏感;ｌｅｕｐｅｐｔｉｎ,ｃｈｙｍｏｓｔａｔｉｎ,ｐｅｐｓｔａｔｉｎ,ａｐｒｏ－ｔｉｎｉｎ,ｐｈｅｎｙｌｍｅｔｈｙｌｓｕｌｆｏｎｙｌｆｌｕｏｒｉｄｅ（ＰＭＳＦ）和ｄｉｔｈｉｏｔｈｒｅｉｔｏｌ（ＤＴＴ）对ｕＣＦ没有影响;ｐｅｐ－ｓｔａｔｉｎ能增强ＣＦＰｇ和ｕＣＦＰｇ活性,Ｅ－６４（一种巯基抑制剂）能增强ｕＣＦＰｇ和ｕＣＦ活性．这些现象说明不能简单将ｅ－ＰＡ归结为丝氨酸蛋白酶或巯基蛋白酶．此外又以纤溶酶原为底物,分析了ｅ－ＰＡ在体外降解天然蛋白质的肽键特异性,结果表明：ｅ－ＰＡ可以切割碱性氨基酸,小的中性氨基酸及Ｍｅｔ的羧基端,同时ｅ－ＰＡ确能将纤溶酶原切割为纤溶酶;这一结论为ｅ－ＰＡ有可能成为新型溶栓药物提供了生化基础．     

麻蝇幼虫肠道类胰蛋白酶的分离纯化及性质(英文)

麻蝇幼虫肠液经硫铵沉淀, ＤＥＡＥ－Ｓｅｐｈａｄｅｘ Ａ－２５离子交换层析, ＳＢＢＩ－Ｓｅｐｈａｒｏｓｅ ４Ｂ亲和层析,分离纯化出一种分子量为 １６ｋＤ的蛋白酶。底物及抑制剂的特异性表明,该酶为类胰蛋白酶。其能够强烈地降解蛋白酶非专一底物酪蛋白和 Ｈｉｄｅ ｐｏｗｄｅｒ ａｚｕｒｅ,以及类胰蛋白酶专一底物 Ｂｚ－Ｐｈｅ－Ｖａｌ－Ａｒｇ ＮＡ, Ｂｚ－Ｐｒｏ－Ｐｈｅ－Ａｒｇ ＮＡ和Ｂｚ－Ｖａｌ－Ｇｌｙ－Ａｒｇ ＮＡ．该酶又能被丝氨酸蛋白酶抑制剂ＰＭＳＦ,类胰蛋白酶抑制剂 ＳＢ－ＢＩ和Ｌｅｕｐｅｐｔｉｎ强烈地抑制。蛋白酶在酸性环境下极不稳定,在弱碱环境（ｐＨ８．５－９．５）中活性最高。     

慈菇蛋白酶抑制剂通过花粉管途径对小麦的导入及转基因植株分析

慈菇蛋白酶制剂（ＡｒｒｏｗｈｅａｄＰｒｏｔｅｉｎａｓＩｎｈｉｂｉｔｏｒ,ＡＰＩ）是来源于慈菇（Ｓａｇｉｔｔａｒｉａｔｒｉｆｏｌｉａ）储藏器官的一种天抗虫物质,属于丝氨酸蛋白酶抑制剂类,能抑制胰蛋白酶、胰凝乳蛋白酶和激肽释放酶,对某些鳞翅目,双翅目以及鞘翅目等昆虫有毒杀作用。     

Expression of the Helicoverpa cathepsin B-like proteinase during embryonic development

Cathepsin B-like proteinase from Helicoverpa armigera (HCB) was proposed as being involved in the degradation of yolk proteins during embryonic development. Recombinant HCB was expressed as a fusion protein with GST in Escherichia coli BL21 on the basis of its cDNA and purified to homogeneity. The fusion protein was cleaved with thrombin to generate a soluble protease with a mass of 37 kDa. A polyclonal antiserum against this recombinant protein, raised in the rabbit, recognized three isoforms of HCB in an ovary homogenate of this insect. Expression of this enzyme during embryonic development was studied using immunoblotting, immunohistochemistry and activity assay. It was found that HCB was expressed during embryonic development and that its proteolytic activity was detected from embryonic developmental eggs. The fact that HCB activity is observed in ovaries and developing eggs suggested that the enzyme had already been activated before embryonic development. Immunohistochemistry indicated that the enzyme was located in follicular cells, the sphere of yolk granules, and the fat bodies of female adult. These lines of evidence suggested strongly that HCB takes part in the degradation of yolk proteins during the development of embryo.     

26S multicatalytic proteinase complexes decrease during the differentiation of murine erythroleukemia cells.

Changes in multicatalytic proteinase activity during differentiation were investigated using Me2SO-induced differentiation of murine erythroleukemia cells as a model. The apparent ATP-dependent multicatalytic proteinase activity decreased in the Me2SO-treated cells with ATP-dependent incorporation of [3H]diisopropyl fluorophosphate decreasing notably after Me2SO-treatment. This decrease in activity does not seem to arise from a cessation of cell-proliferation, because no significant changes in proteinase activity were observed under different culture conditions. Hydroxyapatite column chromatography was employed to analyze the form of multicatalytic proteinase. It was clearly demonstrated that the 26S form of the proteinase decrease in the differentiated cells relative to normal cells. Multicatalytic proteinase-associated proteins that bind to the proteinase in an ATP-dependent manner were purified on an anti-multicatalytic proteinase IgG conjugated column. Only a small amount of protein was recovered from the differentiated cells. These results suggest that the decrease in multicatalytic proteinase-associated proteins that occurs upon cell-differentiation abolishes the ATP-dependent activity of the proteinase.     

Purification and characterization of two distinct Ca2+-activated proteinases from hearts of hypertensive rats

Two distinct Ca2+-activated proteinases were purified and characterized from hearts of hypertensive rats. Ca2+-activated proteinases I and II, having low and high Ca2+ requirements, respectively, were first separated by DEAE-cellulose chromatography. The enzymes were then purified individually by different column procedures: chromatography on phenyl-Sepharose, then Sephadex G-200 for proteinase I and reactive-red agarose for proteinase II. The apparent molecular weight of purified proteinase I was 125 000 and that for purified proteinase II was 110 000. Both enzymes are heterodimers made up of a larger catalytic subunit and a smaller subunit devoid of proteinase activity. Ca2+ concentrations for half-maximal activation were 5 microM for proteinase I and 200 microM for proteinase II. Both enzymes were inhibited by sulfhydryl-modifying agents, but exhibited different characteristics in the auto-digestion reaction in the presence of Ca2+. Proteinases I and II were also purified from hearts of normotensive rats and shown to be identical to their respective counterparts from hearts of hypertensive rats. However, proteinase II activity in hypertensive rat hearts was significantly elevated as compared to controls.     

The primary structure of histone H3 from wheat

Wheat embryo histone H3 has been isolated and purified and the elucidation of the complete amino-acid sequence is described. Peptides were generated by cleavages with CNBr, S. aureus V8 proteinase, endoproteinase Lys-C and trypsin. The peptides were purified by HPLC and the sequence determined by solid-state and gas-phase sequencing methodology. The amino-acid sequence of the protein is identical to pea embryo histone H3 and the sequence deduced from the nucleotide sequence of a wheat embryo histone gene (Tabata T. et al. (1984) Mol. Gen. Genet. 196, 397-400).     

Localization of the proenzyme form of the vitellin-processing protease in Blattella germanica by affinity-purified antibodies

During Blattella germanica embryo development, the nutritive yolk protein vitellin is processed by a cysteine protease, which is activated proteolytically from a proprotease during acidification of yolk granules. A murine polyclonal antiserum was generated with the purified proprotease as the immunogen. The antiserum was made monospecific to proprotease by subtractive affinity chromatography using proprotease-free yolk proteins as ligand. The purified antibodies were employed to investigate the temporal and spatial expression of the proprotease during vitellogenesis and embryo development. Anti-proprotease-reactive peptides appeared in extracts of fat bodies and ovarian follicles of post-mating females, but not in fat bodies of males or the fat bodies or follicles of unmated females, suggesting that the proprotease is synthesized extraovarially. Use of the antibodies was extended to monitor the kinetics of proprotease disappearance during early embryo development. Arch. Insect Biochem. Physiol. 38:109–118, 1998. © 1998 Wiley-Liss, Inc.     

Presence of Active and Inactive Molecules of a Cell Wall-Associated Proteinase in Lactobacillus helveticus CP790

Monoclonal antibodies against a cell wall-associated 45-kDa proteinase from Lactobacillus helveticus CP790 were prepared and used for an immunoblotting analysis of the cell wall extract of CP790. They were found to react with an unidentified 46-kDa protein as well as the 45-kDa proteinase. The 46-kDa protein was copurified with the 45-kDa proteinase by affinity column chromatography using antibody-fixed Sepharose and sodium dodecyl sulfate-polyacrylamide gel electrophoresis and then extracted from the gels. An elution profile of the cyanogen bromide digest of the purified 46-kDa protein obtained by reversed-phase high-performance liquid chromatography was identical to that of the 45-kDa proteinase except for one peak. An analysis of the N-terminal 21-amino-acid sequence revealed that the 46-kDa protein possesses an extra 7 amino acids at the N terminus of the 45-kDa proteinase. The 46-kDa protein was produced at constant levels during fermentation in a skim milk medium, while the 45-kDa protein was mainly observed in the middle of the exponential phase of growth and was produced in proportion to the proteinase activity. Moreover, only the 46-kDa protein was detected in the crude extract of L. helveticus CP791, a variant strain of CP790 defective in proteinase activity. These data strongly suggest that the 46-kDa protein is a precursor, inactive form of the 45-kDa proteinase.     

Purification and characterization of proteolytic enzymes of Leishmania mexicana mexicana amastigotes and promastigotes

Leishmania mexicana mexicana amastigote and promastigote soluble proteinases were purified using gel filtration and ion exchange chromatography. For the amastigotes, two main proteinase activity peaks were separated with both methods. These accounted for approximately 10% and 90% of the total activity. Characterization of the two activities for substrate specificity and sensitivity to inhibitors indicated that the major peak from both column methods contained enzymes with the characteristics of cysteine proteinases. SDS-polyacrylamide gel electrophoresis of the enzyme from the major peak purified by gel filtration revealed one polypeptide with a molecular weight in the region of 31 000. In contrast, the activity of the minor peak eluted from the columns was of higher molecular weight (67 000) and was similar to metalloproteinases. Purification of the soluble proteinases in the promastigote of L. m. mexicana produced only one activity peak from both column techniques. This activity (mol. wt 67 000) corresponded to the high molecular weight proteinase of the amastigote. The purified proteinases were active on 4-nitroanilide and 7-amino-4-methylcoumarin derivatives of various small peptides. The high molecular weight proteinases of both amastigotes and promastigotes were similarly active against most of the peptides, suggesting a low specificity of the enzymes. In contrast, the low molecular weight amastigote proteinases were particularly active against two of the substrates, namely BZ-Pro-Phe-Arg-Nan and Z-Phe-Arg-MCA. These results indicate that a highly active, substrate-specific, soluble proteinase, with characteristics of a cysteine proteinase, is produced upon transformation of the L. m. mexicana promastigote to amastigote. The discovery and characterization of this enzyme offers opportunities for the development of new antileishmanial agents.     

Purification of a neutral proteinase, associated with the actomyosin complex, from uterine myometrium.

We have purified and characterized a neutral proteinase activity from pig uterine myometrium. The proteinase co-purified with the actomyosin complex and could only be separated from it by a high concentration of a chaotropic ion, 3M-NaBr. The proteinase was further purified by gel filtration and affinity chromatography. The purified protein showed a single band on sodium dodecyl sulphate/polyacrylamide-gel electrophoresis corresponding to an Mr of 28 000. Gel filtration on Sephadex G-100 in a buffer containing 3M-NaBr gave an Mr of 27 500. Without the addition of the chaotropic Br- ion, the proteinase aggregates to high-Mr forms of more than 10(6)Da. The proteinase has optimum hydrolytic activity with casein as substrate at pH 7.5-8.0. The thiol-group-blocking reagents p-chloromercuribenzoate, p-chloromercuribenzenesulphonate and Hg2+, as well as soya-bean trypsin inhibitor and 4-aminobenzamidine, inhibited the proteinase. Other bivalent cations, chelating agents and the serine-specific reagents 7-amino-1-chloro-3-tosylamido-L-heptan-2-one and phenylmethanesulphonyl fluoride were without any effect on proteinase activity. The proteinase degraded myosin very rapidly at a molar ratio of proteinase to myosin of 1:50, concomitant with the rate of loss of the ATPase activity. Compared with myosin, actin was only a poor substrate and was degraded at a much lower rate, even at a high molar ratio of the proteinase to actin.     

Partial purification and characterization of cysteine proteinases from various developmental stages of Paragonimus westermani

1. During development of Paragonimus westermani, larvae develop during migration within the host, and adult worms feed on pulmonary tissues, causing significant pathology in the mammalian host. In this report acidic extracts of various developmental stages (metacercariae and worms at one, two and three months of development) were examined for cysteine proteinase activity. 2. A soluble thiol-dependent proteinase activity with a native molecular weight of approximately 20,000 was isolated and partially purified. 3. The enzymes purified from the various developmental stages of the parasite had maximal activity at acidic pH and showed inhibitor susceptibilities similar to the vertebrate acidic cysteine proteinases. 4. Enzymatic activity was stable at pH 5.0 for at least two days when stored at 4 degrees C. 5. It is suggested that these enzymes may be involved in the nutrition of these parasites and/or during penetration and lysis of the tissues.     

Insulin-degrading neutral proteinases of the plasma membrane of loach liver and embryo cells

Insulin-degrading, Ca2+-activated, neutral proteinases of molecular weight about 150 kDa and 70 kDa were purified from plasma membranes of the loach liver and embryo cells. It was shown that dithiothreitol and cysteine enhanced the enzyme activity, whereas p-chloromercuribenzoate and iodoacetic acid inhibited its level. Incubation of isolated plasma membranes with 5'[gamma 32P]ATP resulted in phosphorylation of these proteinases. The intensity of the process increased under the influence of insulin (100 microU/ml), that correlated with a decrease in the activity of proteinase with molecular weight of 150 kDa and an increase in 70 kDa enzyme activity. The data suggest the existence of common regulatory pathways of insulin degradation in plasma membranes of the loach liver and embryo cells.