蝮蛇抗栓酶的临床新用途

蝮蛇抗栓酶的临床新用途苏佳广西桂林南溪山医院（５４１００２）蝮蛇抗栓酶系从蝮蛇蛇毒中提取的一种酶制剂,具有溶栓、抗凝、扩血管和改善微循环作用,被广泛用于脑、心及周围血管性疾病。近年来,随着对蝮蛇抗栓酶药理学与临床研究的进一步深入,其用途也不断扩展,现...     

何谓“清栓酶”“AT—3”?

編辑同志: 近来我们发现蝮蛇抗栓酶的名目较多,有“清栓酶”,报纸上又见有“AT—3”,到底是不是同一样的产品? 田阳县医院邓有辉我国从蛇毒中提取有效成份制成抗血栓药物目前有三种,即用东北白眉蝮蛇毒制成“东北蝮蛇抗栓酶”江浙蝮蛇毒制成的,“江浙蝮蛇抗栓酶”和用五步蛇毒制成的“去纤酶”。     

蝮蛇抗栓酶在儿科临床中的应用

蝮蛇抗栓酶是从东北陆生白眉蝮蛇毒中提取的一种蛋白酶制剂,目前上已广泛应用于治疗心血管病、脑血管病,周围血管病、五官科疾病等,并取得了可喜的疗效,现将其在儿科临床中的应用总结如下:有关蝮蛇抗栓酶药理作用的研究     

蝮蛇抗栓酶在临床中的新用途

蝮蛇抗栓酶在临床中的新用途赵冠群桂林市医学情报所蝮蛇抗栓酶（Ｓｖａｔｅ,又名清栓酶、去纤酶）是由陆生东北蝮蛇、江浙蝮蛇的蛇毒中提取、分离纯化的蛋白水解酶和精氨酸酶制剂,郝文学等氏业已证实它具有抗凝、溶栓、降脂、去纤、降低血液粘度和血小板聚集、扩张血管...     

蝮蛇抗栓酶治疗皮肤病的临床疗效观察

蝮蛇抗栓酶治疗皮肤病的临床疗效观察石玉芳（贵州省都匀市医院综合科５５８０００）蝮蛇抗栓酶（清栓酶）是由东北陆生白眉蝮蛇中提取的一种酶制剂,主要用于脑血栓病的防治。用于治疗皮肤病的报道甚少。笔者从１９９１年６月～１９９５年３月。用清栓酶治疗皮肤病１０３...     

蝮蛇抗栓酶的不良反应及注意事项

蝮蛇抗栓酶的不良反应及注意事项尤荣开浙江省温州市第二医院神经内科３２５０００蝮蛇抗栓酶是从蝮蛇蛇毒中提取的酶制剂,含有十几种不同刺激因子,具有类凝血酶的抗凝作用,临床广泛应用于脑心血管疾病的治疗,随着临床研究的深入,各种杂志陆续报道一些不良反应,为引...     

蝮蛇抗栓酶－Ⅲ大剂量冲击疗法治疗脑血栓52例报告（摘要）

蝮蛇抗栓酶－Ⅲ大剂量冲击疗法治疗脑血栓５２例报告（摘要）抚顺市新抗区人民医院张亚杰,张明慧本文报告应用蝮蛇抗栓酶－Ⅲ大剂量冲击疗法治疗７２小时内发病的急性脑血栓５２例,并与低分子右旋糖酐加维脑路通治疗对照组５０例观察。治疗方法：第一天用抗栓酶Ⅲ２．５...     

蝮蛇抗栓酶的不良反应

蝮蛇抗栓酶的不良反应张海燕广西南宁市第二人民医院５３００３１蝮蛇抗栓酶（Ｓｖａｔｅ）是从蝮蛇毒中提取的酶制剂,是临床上常用的抗凝剂。近年来由于在医疗工作中广泛使用,其不良反应越来越多,现将其不良反应综述如下,以期临床用药时注意。１心血管系统反应杨菊贤...     

关于精制蝮蛇抗栓酶的问答

于1991年5月下旬在昆明召开的中国蛇毒酶临床应用研讨会后,陆续收到许多读者来信,询问精制蝮蛇抗栓酶有关问题。为了能较全面地回答读者来信,采访了有关专家并做了某些调查,对几个共同问题公开做答,不专门复信,见谅。一、精制蝮蛇抗栓酶的本质是什么?答:根据昆明会议信息。精制蝮蛇抗栓酶就是原来的“江浙蝮蛇毒抗栓酶-3号”,由中国医科大学老年病防治中心在沈阳第一制药厂生产的江浙蝮蛇抗栓酶(Svate)基础上,经过两次分离所得的产物。经过动物实验及临床验证认为:毒副反应明显低于原江浙蝮蛇抗栓酶。为了区别于原江浙蝮蛇抗栓酶,已被辽宁省卫生厅批准正式批量生产。商品名称为“精制蝮蛇抗栓酶”。为什么要取消“江浙”二字,其     

蝮蛇抗栓酶与精制蝮蛇抗栓酶制剂的比较研究

本文作者对以东北长白山白眉蝮蛇毒为原料生产的两种酶制剂——蝮蛇抗栓酶与精制蝮蛇抗栓酶进行了比较研究。用 HPLC 柱层析粗毒得到15个蛋白峰,同时对两种酶制剂以 HPLC 层析用两根层析柱串联上样层析以提高其分辩率,得到两个图谱,蝮蛇抗栓酶有7个蛋白峰,而精制品有3～4个蛋白峰.同时以 SDS-PAGE 电泳图谱.蝮蛇抗栓酶呈现7～8条谱带,精制品有4～5条谱带,并与已知分子量的标准蛋白进行对比,结果表明两种酶制剂均非单一组分.蝮蛇抗栓酶谱带较多,精制品较纯.其分子量均在2～6万之间.蝮蛇抗栓酶几个组分有协同作用,每次剂量在0.25～0.50单位,即有明显疗效,而精制品临床用药剂量较大,每次0.75～1.0单位,多者达1.25单位(3～5支).     

Revision of Maranta subgen. Maranta (Marantaceae)

Maranta subgen. Maranta includes species related to M. arundinacea L. It is characterized by aerial shoots with a strong monopodial tendency, absence of root tubers, simple inflorescences or few-branched, often diffuse synflorescences, florescences with few, herbaceous spathes, and comparatively large, distinctly pedicellate flowers. There are occasional exceptions to all these characters. Most species are partial selfers, only two or three being allogamous. Sixteen species are recognized, eight of which are new: M. linearis, M. sobolifera, M. lindmanii, M. zingiberina, M. incrassata, M. rupicola, M. amazonica , and M. tuberculata. The new species are described, and all species are defined and discussed, data being given about distribution and habitat. Growth habit and rhizome structure are essential taxonomic characters, but leaf shape and indument distribution are more useful characters for routine identification. Of the species referred to subgen. Automaranta by Schumann in Das Pflanzenreich, three are excluded: M. cordata, M. pohliana , and M. foliosa.     

Synthesis and biological activity of 7,8-dihydro derivatives of batrachotoxinin interacting with fast sodium channels

7,8-Dihydrobatrachotoxinin (A) (I) was synthesized from 11 alpha-hydroxyprogesterone (III) by a 37-stage procedure. Trimethylpyrrolcarboxylate, benzoate as well as 2-azido-benzoate derivatives of (I) were obtained by mixed anhydride technique, the latter two derivatives being prepared also with tritium atoms in aromatic rings (sp. radioactivity about 28 Cu/mmol). Upon interaction with rat brain synaptosomes the apparent Kd of 7,8-dihydrobatrachotoxinin A 20 alpha-[4-3H]benzoate (Iv) was about 2,5 x 10(-6) M. The (Iv) specific binding was inhibited by aconitine with K0,5 = 1,3 x 10(4) M. Anemonia sulcata toxin II (ATX II) enhanced (Iv) affinity for the receptor up to 7 x 10(-7) M, the maximum binding capacity being 2,5 pmol/mg of protein. Benzocaine and tetracaine competitively displaced specifically bound toxin with K0,5 = 3,1 x 10(-4) M and 5,7 x 10(-7) M, respectively, in the presence of 10(-5) M ATX II. 2-Azido[5-3H]benzoate derivative (Id) was shown to be an effective probe for covalent labeling of the alkaloid toxin receptor of the sodium channel.     

结核分枝杆菌基因组学与基因组进化

在后基因组时代,特别是在新的测序理论和设备大发展的背景下,一些重大传染性致病微生物基因组序列正在被逐一测定,并且随后的基因功能注释,蛋白质三维结构重建等工作也正在开展,以期对致病微生物的生物学特性、诊断策略和治疗方法等有突破性的认识.作为对人类健康一直存在严重威胁的结核分枝杆菌,其基因组在进化中所发生的各种遗传事件对其生物学性质、致病能力和抗药性等各方面有重要作用.本文旨在阐述结核分枝杆菌的起源及其基因组特征,论述其基因组进化的研究进展.     

Studies on the Scutellar Bristles of DROSOPHILA MELANOGASTER. II. Long-Term Selection for High Bristle Number in the Oregon Rc Strain and Correlated Responses in Abdominal Chaetae

Results are presented of 135 generations of selection for high scutellar bristle number in two lines M and M3 derived from the same original mating of one female with 5 bristles by one male with 4 bristles, the latter being the wild-type canalised phenotype. Results are also given of two relaxed lines per line and of a reselection line M2 derived from the first relaxed line of line M which had regressed almost to base population level. The effect of introducing the sc(1) allele into the M and M3 selected backgrounds was studied at generations 39-44. At the end of selection the effect of an extra dose of sc(+) was also studied in males of all selected backgrounds. The correlated responses in abdominal bristles were followed in all lines.-Considering their common origin, the selection lines differed markedly in pattern of scutellar response and in most other aspects observed, namely correlated responses in abdominals and p.c. scutellars, sex differences, and behaviour on relaxation. Selection limits for scutellar bristles in lines M and M2 were equal to or greater than the most extreme reported in the literature.-The probit span of the canalised 4 bristle class decreased in each selection line as the mean scutellar bristle number increased, and increased again in the relaxed lines as the mean bristle number decreased. In the context of an hypothesis that canalisation at 4 bristle is due to regulation of the scute locus, this result is now interpreted as being due mainly to selection for poor regulators of sc(+), in contrast to a previous interpretation that only the minor gene background was altered by selection, the canalisation (regulation) genotype not being affected.-Introducing the sc(1) allele into the selected backgrounds M and M3 showed a reduced effect on sc(1) flies compared with sc(+) flies, and an interaction of sc(1) and sc(+) with selected background. sc(1) flies had about the same number of bristles in both backgrounds though the mean of sc(+) flies in line M was about 3sigma higher than in line M3. Dominance of sc(+) to sc(1) was reduced slightly in M3. However, the effect of an extra dose of sc(+) at the end of selection was about the same as in unselected in all lines, so the first or dominance level of regulation of the scute locus was not significantly affected by selection, though the second or canalisation level of regulation was.-A large positive correlated response in abdominal bristles occurred in all lines. The response in line M was about twice that in M2 and M3 and was in fact as large as can be obtained from direct selection on abdominals. In line M some genes may have been selected with a proportionately greater effect on abdominals than on scutellars. This is supported by the further observation in line M that the abdominal scores of flies with particular scutellar bristles scores increased as the scutellar mean increased. An attempt was made to apply to these results Rendel's (1962) model of competition between scutellars and abdominals for common bristle-making resources. This could not be done satisfactorily mainly because the assumptions in the model about the similarity of effects in scute and wild-type flies were not met in the present material.     

Characterization of the denatured states distribution of neocarzinostatin by small-angle neutron scattering and differential scanning calorimetry

The denatured states of a small globular protein, apo-neocarzinostatin (NCS), have been characterized using several techniques. Structural properties were investigated by optical spectroscopy techniques and small-angle neutron scattering (SANS), as a function of guanidinium chloride (GdmCl) concentration. SANS experiments show that in heavy water, the protein keeps its native size at GdmCl concentrations below 2.5 M. A sharp transition occurs at about 3.6 M GdmCl, and NCS behaves like an excluded volume chain above 5 M. The same behavior is observed in deuterated buffer by fluorescence and circular dichroism measurements. For the H(2)O buffer, the transition occurs with lower concentration of denaturant, the shift being about 0.6 M. 8-Anilino-1-naphthalenesulfonate (ANS) was used as a hydrophobic fluorescent probe for studying the early stages of protein unfolding. Protein denaturation modifies the fluorescence intensity of ANS, a maximum of intensity being detected close to 2 M GdmCl in hydrogenated buffer, which shows the existence of at least one intermediate state populated at the beginning of the unfolding pathway. Differential scanning calorimetry (DSC) was used to obtain thermodynamic values for NCS denaturation. The melting curves recorded between 20 and 90 degrees C in the presence of various GdmCl concentrations (0-3 M) cannot be explained by a simple two-state model. Altogether, the data presented in this paper suggest that before unfolding the protein explores a distribution of states which is centered around compact states at denaturant concentrations below 2 M in H(2)O, and then shifts to less structured states by increasing denaturant concentrations.     

基于Pacbio第三代测序技术的厚朴基因组测序分析

厚朴为著名的传统药用植物,归于木兰科、木兰属,于我国广泛种植,其树皮、根皮、枝皮、叶片、花、果实均能入药或食用。为获取厚朴全基因组序列信息,该文以厚朴叶片DNA为材料,采用Pacbio Sequel第三代测序技术构建厚朴全基因组数据库,并利用生物信息学方法对获得的核苷酸序列进行组装、功能注释以及进化分析研究。结果表明:(1)原始测序数据过滤后获得140.91 Gb三代数据,Read N50约为13 784bp,经过组装得到厚朴基因组大小为1.68 Gb,Contig N50约为222 069 bp,单拷贝基因完整性为81.0%。(2)组装后的序列通过与NR、KOG、KEGG等功能数据库比对,共有98.40%的基因得到了功能注释,其中KOG功能注释结果发现厚朴的蛋白功能主要集中在一般功能预测、翻译后修饰、蛋白质转换、伴侣以及信号转导机制; GO功能分类表明厚朴的基因集中在细胞组分及生物学过程; KEGG分析发现厚朴参与代谢通路的基因占主要地位。(3)通过与葡萄、拟南芥、水稻、杨树、银杏、无油樟、茶树及牛樟基因组的比对分析,发现厚朴23 424个基因中有20 801个基因可以分类到12 129个家族,其中有515个基因家族为厚朴所特有,而厚朴与牛樟(樟科)亲缘关系较近,两者的分化时间约在122.5百万年前(mya)。该研究首次利用第三代测序技术对厚朴全基因组解析,有利于对其进一步进行深入的开发与利用,也为研究其他药用植物全基因组奠定了基础。     

Extraction and fractionation of proteoglycans from squid skin

The extractability of squid skin proteoglycans with solutions of varying concentrations of guanidine-HCl, urea and SDS was studied; 4 M guanidine-HCl, being the best extractant, removed 95% of the tissue proteoglycans (glycosaminoglycan uronic acid). The proteoglycans in the 4 M guanidine-HCl extract were fractionated by repeated ion exchange and gel chromatography on Sepharose CL-4B to give three main populations, all being present in about equal proportions. Two populations (Kd 0.34 and 0.56) contained only chondroitin (proteochondroitin) and the other (Kd 0.50) only oversulphated chondroitin sulphate (oversulphated proteochondroitin sulphate). Two minor populations, one containing chondroitin and chondroitin sulphate and the other chondroitin sulphate and oversulphated chondroitin sulphate, were also identified.     

The patterning of compensatory sugar feeding in the Australian sheep blowfly

Abstract. The pattern of feeding is described for males of the Australian sheep blowfly, Lucilia cuprina , with ad libitum access to either 0.1 M or 1.0 M glucose solution. Flies given the 0.1 M solution ingested nearly 3 times the volume taken by flies given the 1.0 M solution by eating meals of, on average, twice the size about 1.5 times as frequently. Flies were usually relatively inactive following a meal, with the extent of this post-prandial quiescence being a function both of meal size and concentration of sugar. Quiescence lasted only about 20% of the average intermeal interval, however, and there was no correlation between meal size and time to the next meal. The crop emptied more slowly when it contained 1.0 M rather than 0.1 M glucose solution and the crop was, on average, fuller at the beginning of a meal on the higher concentration. The volume of solution imbibed during a meal was positively correlated with time since the end of the preceding meal. The average crop volume at the end of a meal was similar in flies feeding on 0.1 M and 1.0 M solutions. The results are considered in relation to published information on control of feeding and compensation in the blowfly Phormia regina.     

Transplacental transport of alpha 2-macroglobulin (alpha 2M) and induction of alpha 2M in maternal and neonatal rats with acute inflammation.

The aims of this study were to investigate transplacental transport of alpha 2-macroglobulin (alpha 2M) in rats in rats and to examine the degree of alpha 2M induction in maternal and neonatal rats with acute inflammation. Serum was collected from healthy pregnant CD (IGS) rats, neonates of the pregnant rats and their cord blood. Additional serum samples were obtained from pregnant rats inoculated with an inflammatory agent, turpentine oil, their neonates and cord blood, and neonates inoculated with turpentine oil. The serum levels of alpha 2M were measured by means of an enzyme-linked immunosorbent assay. The average serum levels of alpha 2M in healthy neonates and cord blood were about 380 micrograms/ml. Serum a2M level in neonates inoculated with turpentine oil averaged about 580 micrograms/ml. Serum alpha 2M levels in maternal rats inoculated with turpentine oil, neonates from those rats and their cord blood were elevated, the values being 2,000 micrograms/ml or higher. It was demonstrated that induction of alpha 2M in neonatal rats was lower than in maternal rats when inoculated with turpentine oil. These results suggest that alpha 2M is transplacentally transported from maternal rats to fetal ones.     

Spin echo proton NMR studies of the metabolism of malate and fumarate in human erythrocytes: Dependence on free NAD levels

The NAD-dependent conversion of malate to lactate in human erythrocytes was studied by spin echo proton NMR. A pathway involving the decarboxylation of oxaloacetate catalysed by haemoglobin is proposed to account for the observed reaction. NADP-dependent reaction was negligible. The rate of the reaction was measured in intact erythrocytes under controlled conditions. This rate correlates with that obtained with lysates at 30 μM free NAD and that obtained with purified human erythrocyte enzymes at about 15 μM NAD. The total extractable NAD in the intact cells was 70–90 μM. Experiments with cells containing elevated NAD levels could be explained by a significant fraction of the NAD being weakly bound (K_d about 1 mM) to haemogloin.