透明质酸酶的研究进展

透明质酸酶是以降解透明质酸为主的糖苷酶。近年来国内外关于透明质酸酶各方面的研究日益增多,透明质酸酶的构效关系及生物学应用越来越引起人们的关注。对透明质酸酶的相关研究进行了综述,主要阐述了各类型透明质酸酶的研究概况包括人透明质酸酶、牛睾丸透明质酸酶、毒液透明质酸酶、微生物透明质酸酶。简要介绍了透明质酸酶的活性测定、酶活抑制剂及透明质酸酶制剂的应用情况,最后对透明质酸酶的研究前景进行展望。     

山茱萸抗过敏活性组分的筛选及其对RBL-2H3细胞脱颗粒的作用CSCD

为研究山茱萸中抗过敏活性成分,采用透明质酸酶抑制实验对山茱萸中活性组分进行初步筛选;采用细胞脱颗粒抑制实验对透明质酸酶抑制活性较高的组分进一步评估;采用气相色谱-质谱联用法(GC-MS)进行成分分析。结果表明山茱萸石油醚部位(petroleum ether extract of Corni Fructus,COPE)具有显著透明质酸酶抑制活性,其IC50值为3.11 mg/mL;经硅胶柱层析分离得到4个透明质酸酶抑制活性更高的组分,其中组分COPE-8对RBL-2H3细胞脱颗粒抑制作用更显著,呈剂量依赖形式且具低细胞毒性。经20μg/mL COPE-8处理后,RBL-2H3细胞脱颗粒释放的组胺和β-氨基己糖苷酶分别减少46%和39%;经GC-MS分析,COPE-8中主要活性物质为萜类物质,包括α-香树脂醇、β-香树脂醇和香紫苏醇。结果表明COPE-8具有显著的抗过敏活性,在抗过敏活性物开发方面具有一定的应用价值。     

透明质酸酶的研究进展

透明质酸酶是能降解透明质酸及部分糖胺聚糖的一类糖苷酶,可应用于医疗和美容等领域。透明质酸酶也可用于制备小分子糖胺寡糖,许多研究发现小分子糖胺寡糖具有比大分子糖胺聚糖更高的生物免疫活性。为便于研究人员对透明质酸酶进行进一步的基础研究及应用研究,本文介绍了透明质酸和透明质酸酶,梳理了透明质酸酶的分类、结构和催化机理,归纳总结了透明质酸酶的酶活力测定方法、重组表达、酶学性质和应用,展望了透明质酸酶的研究方向。     

金黄色葡萄球菌透明质酸裂解酶HylS的异源表达与特性研究

透明质酸酶能够将透明质酸聚糖降解成具有抗氧化等生物活性的低分子量寡糖.微生物来源透明质酸酶具有酶学性质多样和易于重组表达等特点,是开发透明质酸酶的研究热点.通过基因组测序获得一个潜在的金黄色葡萄球菌来源透明质酸裂解酶基因hylS,将其进行了大肠杆菌BL21(DE3)异源重组表达,并对重组酶进行了酶学特性和酶解产物抗氧化...     

舒敏中药提取物制备及其功效评价研究CSCD

本文对香薷、山慈菇、独活、三棱、孩儿茶、远志六味中药进行提取,采用抑制透明质酸酶活性、清除自由基、抑制组胺释放实验来验证组方提取物的活性,并将其添加到乳液配方中,进行舒敏功效评价。结果表明:质量分数为6%的组方提取物对透明质酸酶抑制率达80.06%,对超氧阴离子自由基、羟自由基、DPPH自由基清除率均在70%以上;浓度为200μg/mL的组方提取物抑制组胺释放率达52%,这表明组方提取物对透明质酸酶、组胺释放及三种自由基均有一定的抑制或清除作用。人体功效评价结果表明,添加了组方提取物的乳液能够显著减少皮肤血红素(P<0.01),减少皮肤水分散失(P<0.01),提高皮肤水分含量(P<0.01),这表明该乳液能有效舒缓皮肤过敏症状,增强皮肤屏障功能。     

一株产透明质酸酶的菌株鉴定及酶学性质研究

透明质酸酶可用于药物渗透剂、动物皮革松散及低分子量的透明质酸制备.实验室前期筛选了一株具有较高透明质酸降解能力的菌株,本研究对其进行了 16S rRNA基因和生理生化反应鉴定,鉴定为弗氏柠檬酸杆菌,但弗氏柠檬酸杆菌来源的透明质酸酶的功能还未见报道.因而,以透明质酸为底物研究其酶学性质,结果表明:该酶最适pH值为5.5,在pH值4.0～8.0下处理1 h可以保持60％以上酶活力;最适温度为50℃,在50℃和60℃下处理1h后剩余60％以上的酶活力.该酶和人源透明质酸酶最适pH相似,但其耐热性更高.因此,本研究挖掘到了新颖的透明质酸酶的资源,并为其开发利用提供了参考价值.     

关于水蛭透明质酸酶的研究

关于水蛭透明质酸酶的研究杨潼（中国科学院水生生物研究所武汉４３００７２）关键词水蛭，透明质酸酶，提取物透明质酸酶（Ｈｙａｌｕｒｏｎｉｄａｓｅ）这个词最初是用来命名从动物组织中得到的能水解透明质酸的酶，后来人们发现这个命名并不恰当，因为从许多动物体内得...     

黄唇蜾赢蜂蜂毒中两个过敏原全长基因的克隆、序列分析和表达

为了进一步研究透明质酸酶的过敏活性,利用昆虫杆状病毒成功地表达了黄唇蜾赢蜂Rhynehium brunneum蜂毒的透明质酸酶。根据已报道的胡蜂科透明质酸酶和抗原5基因的氨基酸保守序列,设计合成简并引物,利用反转录多聚酶链式反应（RT—PCR）技术扩增了黄唇蜾赢蜂蜂毒透明质酸酶和抗原5的基因片段,利用RACE技术进一步获得了它们的全长基因（GenBank登录号分别为EU624135和EU624136）。按照过敏原的命名法则,分别命名为Rhyb2和Rhyb5。序列比对分析发现,这两个基因与胡蜂科的相应序列高度相似,说明对胡蜂蜂毒过敏的人群也可能对蜾赢蜂蜂毒有交叉过敏反应。但进一步分析发现,黄唇蜾赢蜂蜂毒透明质酸酶的B细胞决定表位显著不同,9个保守性氨基酸在蜾赢蜂中仅保留了3个,而且缺乏两个关键的精氨酸;黄唇蜾赢蜂蜂毒抗原5序列N端的二级结构和具有过敏活性的常见黄胡蜂Vespula vulgaris蜂毒的抗原5显著不同,有可能因此而缺失依赖其N端二级结构的B细胞决定表位。据此认为,蜾赢蜂蜂毒透明质酸酶和抗原5很可能是天然弱化的过敏原,在过敏原特异性免疫治疗上具有潜在的应用价值。     

黄唇蜾蠃蜂蜂毒中两个过敏原全长基因的克隆、序列分析和表达

为了进一步研究透明质酸酶的过敏活性,利用昆虫杆状病毒成功地表达了黄唇蜾蠃蜂Rhynchium brunneum蜂毒的透明质酸酶。根据已报道的胡蜂科透明质酸酶和抗原5基因的氨基酸保守序列,设计合成简并引物,利用反转录多聚酶链式反应（RT-PCR）技术扩增了黄唇蜾蠃蜂蜂毒透明质酸酶和抗原5的基因片段,利用RACE技术进一步获得了它们的全长基因（GenBank登录号分别为EU624135和EU624136）。按照过敏原的命名法则,分别命名为Rhy b 2和Rhy b 5。序列比对分析发现,这两个基因与胡蜂科的相应序列高度相似,说明对胡蜂蜂毒过敏的人群也可能对蜾蠃蜂蜂毒有交叉过敏反应。但进一步分析发现,黄唇蜾蠃蜂蜂毒透明质酸酶的B细胞决定表位显著不同,9个保守性氨基酸在蜾蠃蜂中仅保留了3个,而且缺乏两个关键的精氨酸;黄唇蜾蠃蜂蜂毒抗原5序列N端的二级结构和具有过敏活性的常见黄胡蜂Vespula vulgaris蜂毒的抗原5显著不同,有可能因此而缺失依赖其N端二级结构的B细胞决定表位。据此认为,蜾蠃蜂蜂毒透明质酸酶和抗原5很可能是天然弱化的过敏原,在过敏原特异性免疫治疗上具有潜在的应用价值。     

透明质酸生物合成途径及基因工程研究进展

透明质酸是由N-乙酰氨基葡萄糖和葡萄糖醛酸组成的双糖单位聚合而成的直链酸性黏多糖,已被广泛应用于药物、化妆品和食品添加剂。微生物发酵法是目前生产透明质酸最有效的方法。生物体内透明质酸的合成途径基本一致,均为Leloir途径。透明质酸合成操纵子由透明质酸合酶基因、尿苷二磷酸葡萄糖脱氢酶基因和尿苷二磷酸葡萄糖焦磷酸化酶基因组成,其表达受Cov S/CovR和Lux S等多种调控系统调控。随着分子生物学技术的迅速发展以及对透明质酸合成相关基因了解的不断深入,人们从提高透明质酸安全性、提高透明质酸产量和调控透明质酸分子质量三个方面出发,通过基因工程手段构建出了高产、安全、一定分子质量范围的透明质酸生产菌株。就有关透明质酸生物合成途径、合成相关基因表达调控及生产菌株分子生物学改造的策略与研究进展进行综述和展望。     

Snake venom hyaluronidase: a therapeutic target

The diffusion of toxins from the site of a bite into the circulation is essential for successful envenomation. Degradation of hyaluronic acid in the extracellular matrix (ECM) by venom hyaluronidase is a key factor in this diffusion. Hyaluronidase not only increases the potency of other toxins but also damages the local tissue. In spite of its important role, little attention has been paid to this enzyme. Hyaluronidase exists in various isoforms and generates a wide range of hyaluronic acid degradation products. This suggests that beyond its role as a spreading factor venom hyaluronidase deserves to be explored as a possible therapeutic target for inhibiting the systemic distribution of venom and also for minimizing local tissue destruction at the site of the bite.     

Characterization of lysosomal-type hyaluronidase in the culture medium of 2 cell lines derived from human hepatomas

A sensitive assay for hyaluronidase was developed using as a substrate, hyaluronic acid insolubilized on polystyrene microtest plates. Hyaluronic acid was measured exploiting the fact that it can bind immune complexes made up with hyaluronectin and alkaline phosphatase-conjugated anti-hyaluronectin antibodies. Hyaluronidase was detected in both cell line culture media. Optimum pH was between 3.25 and 3.75. Sodium chloride dependence was absolute, and the optimum concentration of sodium chloride was between 0.2 and 0.3 M. The activity was not affected by dialysis, and was suppressed by a 5 minute heating at 50 degrees C or by protease treatment. The molecular weight was 68 K as determined by gel permeation chromatography. The results are close to those reported for human lysosomal hyaluronidase.     

Proteases from actinomycetes interfere in solid media plate assays of hyaluronidase activity

Four hundred and fifteen actinomycete strains were screened for hyaluronidase activity in two plate assays media. In the first one, using hyaluronic acid as substrate and bovine serum albumin (BSA) to help precipitation of the nondegraded substrate, only strain 594 and hyaluronidase control were positive. In the second assay, plates with hyaluronic acid, but not BSA, gave the same results. For plates containing only BSA, proteinase activity was detected in strain 594. When hyaluronic acid was treated with pronase, the only clear zones, in the second assay without BSA, were those around hyaluronidase controls. Protease activity, commonly found in actinomycetes, was detected only in strain 594, among the 415 studied, when tested in hyaluronidase assay using hyaluronate plus BSA. This may be due to the composition of the growth medium, since media with different composition gave different results for protease activity in each of the 15 strains analyzed. These data suggest that proteases can affect an accurate detection of hyaluronidase in media containing proteins, not only from hyaluronate preparations, but also from other medium ingredients. Thus, for a correct interpretation of the method, they must be excluded. Commercial Hyaluronidase used as controls must be also tested for the presence of protease contamination.     

The Influence of Hyaluronidase and Hyaluronidase Substrates on Penetration of Cultured Cells by Eimerian Sporozoites

SYNOPSIS Leighton tube cultures of bovine embryonic kidney cells were inoculated with Eimeria adenoeides sporozoites suspended in media containing either hyaluronidase, hyaluronidase substrates (chondroitin sulfate and hyaluronic acid) or Ficoll. After 1 hr at 41 C, coverslips were removed and cells were fixed and stained. Hyaluronidase (1 and 10 mg/ml) did not increase the number of intracellular sporozoites. Chondroitin sulfate (1 and 10 mg/ml) and hyaluronic acid (1 mg/ml) did not reduce the number of intracellular sporozoites. However, the number was reduced when the media contained either chondroitin sulfate (100 mg/ml) or hyaluronic acid (5 mg/ml), which were quite viscous.
Ficoll (117 mg/ml), which produced the same viscosity as 5 mg hyaluronic acid/ml, also reduced the number of intracellular sporozoites. This finding circumstantially indicates that sporozoites may be physically inhibited from entering cells by the high viscosity of the substrates.
Biochemical tests, which detected as little as 0.2 μg of known hyaluronidase, failed to detect hyaluronidase activity in excysted intact or fragmented E. adenoeides sporozoites or in sporozoites within E. tenella oocysts.     

Purification and properties of hyaluronidase from bull sperm.

Hyaluronidase from bull sperm was fractionated by ammonium sulfate and further purified by DEAE-cellulose and Sephadex chromatography. The highly purified hyaluronidase preparation showed 2,370 units per mg of protein (68,730 N.F. units per mg of protein), i.e. 182-fold purification. Disc gel electrophoresis showed one major component. The molecular weight of bull sperm hyaluronidase was 62,000 by sodium dodecyl sulfate gel electrophoresis. Hyaluronidase from bull sperm has optimum activity at pH 3.8 and an absolute requirement for cations. Kplus and Naplus have a greater effect than Ca2plus, Mg2plus, and Mn2plus, whereas Co2plus, Cu2plus, and Zn2plus do not affect the enzyme activity. Purified preparations are less stable than crude extracts stored frozen at minus 15 degrees. Km of hyaluronidase with hyaluronic acid as substrate is 3.7 mg per ml and Vmax is 2.4 mumol per min by Hofstee plot.     

Hyaluronic acid is an endogenous inducer of interleukin-1 production by human monocytes and rabbit macrophages

When human peripheral monocytes and rabbit peritoneal macrophages were incubated with hyaluronic acid, the media were found to contain interleukin-1 (IL-1) activity and to stimulate collagenase production by rabbit fibroblasts. A digestion of hyaluronic acid by testicular hyaluronidase decreased the IL-1 inducing activity. Polymixin B, an inhibitor of endotoxin, did not exert any effect towards the action of hyaluronic acid. Hyaluronic acid also stimulated human polymorphonuclear leucocytes to produce IL-1 like activity. These results indicate that hyaluronic acid is an endogenous IL-1 inducer and may play important roles in the pathological and/or physiological changes of connective tissues.     

Isolation, properties, immunological specificity and localization of mouse testicular hyaluronidase

Hyaluronidase (hyaluronate 4-glycanohydrolase, EC 3.2.1.35) was purified from mouse testes by ion-exchange chromatography, Sephadex G-200 filtration and Con A-agarose affinity chromatography. The final preparation had 94-fold purity and 12.2 units spec. act. of the enzyme (unit of specific activity = mumol N-acetylglucosamine released/h per mg protein at 37 degrees C and pH 4.5). Hyaluronidase is relatively heat stable and loses 10-20% of its activity at 50-55 degrees C for 10 min. Ea for eat denaturation of enzyme is 42-45 kcal between 45 an 63 degrees C. The Michaelis constant of mouse testicular hyaluronidase is 1.1 mg/ml hyaluronic acid. Antibodies to the purified enzyme were produced in rabbits and showed a single precipitin line by Ouchterlony gel diffusion. Antiserum to hyaluronidase inhibited enzyme activity by 25%. Immunologically, mouse testicular hyaluronidase is species specific. Tissue extracts of mouse vital organs, except testes and epididymis did not react with the antisera, though nonspecific precipitation occurred between intestinal extracts and anti-hyaluronidase serum. Hyaluronidase was localized in testis sections by indirect immunofluorescence. A specific dark green fluorescence was localized on cell boundaries extending from spermatogonia to spermatids and appeared on the sperm acrosome. Cytoplasm of spermatogonia and spermatocytes showed light green fluorescence, whereas interstitial tissue was devoid of fluorescence.     

Immunoenzymic studies on testicular hyaluronidase from rhesus monkeys (Macaca mulatta)

Hyaluronidase from rhesus monkey testes was purified by detergent extraction, ammonium sulphate fractionation, Sephadex G-200 column chromatography and concanavalin A-Sepharose affinity chromatography. The purified hyaluronidase showed one protein band on acrylamide gel electrophoresis. Antibodies to the purified hyaluronidase were raised in rabbits and showed a single precipitin line by Ouchterlony gel diffusion. The enzyme had a molecular weight of 62,000. The Km was 0.5 mg/ml for hydrolysis of hyaluronic acid at 37 degrees C. The optimum pH for the enzyme was 5.0 but activity was present over a broad pH range. The hyaluronidase was inhibited by HgCl2, CuSO4, FeSO4 and p-chloromercuribenzoate all at a concentration of 2 x 10(-4) M. Cysteine protected the enzyme against HgCl2 inhibition.     

THE HYALURONIDASE OF BRAIN

Abstract— Hyaluronidase (hyaluronate glycanohydrolase, EC 3.2.1.35), with a pH optimum of 3.7, was detected in rat and bovine brain. It degraded hyaluronic acid and, at a slower rate, chondroitin sulphate to a mixture of higher oligosaccharides with N-acetylhexosamine at the reducing end. The enzyme was enriched 5- and 6-fold in a crude lysosomal fraction of rat brain or bovine cerebral cortex, and was further purified to a total enrichment of 9-fold by ammonium sulphate fractionation. The enzyme activity in grey matter was more than twice that found in white matter, and there was no significant change in enzyme activity as a function of increasing age from the neonatal to the adult rat brain. The level of hyaluronidase activity in rat brain is considerably greaterthan that required to account for the rate of catabolism of hyaluronic acid and chondroitin sulphate measured in vivo.     

Inaccessibility of certain Ricinus lectin binding sites due to the increase in hyaluronic acid during chick embryo development

Chick embryo fibroblasts constitute a useful model for investigating cell surface differentiation using Ricinus lectin as a marker. Fibroblasts from 8-day chick embryos had two classes of Ricinus lectin binding sites, whereas those from 16-day embryos displayed only one class. Hyaluronidase treatment of fibroblasts from 8-day embryos had no effect on their capacity to bind Ricinus lectin; however after this treatment, 16-day cells resembled 8-day cells since the former also exhibited two classes of lectin-binding sites. Treatment with hyaluronidase released 2-5 times more hyaluronic acid from the older cells than from the younger cells. The same hyaluronidase treatment did not change the number of 8-day cells detached by trypsin from the substrate, but increased the number of detached 16-day cells. These observations suggest (i) that the greater adhesiveness to the substrate of the 16-day cells might be due to the presence on the cell surface of a larger amount of glycosaminoglycans at 16 days than at 8 days, and (ii) that the increased accumulation of hyaluronic acid on the cell surface might be involved in an alteration in the cell membrane during differentiation.