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1.
用火箭电泳法测定溶菌酶活性 总被引:2,自引:0,他引:2
<正> 测定体液中溶菌酶含量的方法有免疫学和酶学方法两大类。常用的琼脂平板打孔法是一种酶学测定法,其测定范围为10—1000μg/ml。但人和小鼠血清溶菌酶活性分别约为2μg/ml和5μg/ml,低于上述测定范围。因此单用琼脂平板打孔法研究血清溶菌酶活性的细微变化是有困难的。我们将酶学方法和电泳方法结合在一起。由于酶的作用区域增加,灵敏度随之提高。此法类似抗原抗体在电冰过程中形成沉淀的火箭电泳法,但实际上并不是 相似文献
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为选择一种准确快捷的方法测定银耳多糖的单糖组成,对薄层色谱法(TLC)、气相色谱法(GC)、高效液相色谱法(HPLC)三种色谱方法进行比较。结果表明,前两种方法的测定结果均不理想,而HPLC法,操作简便,灵敏度高,分离效果好,信息完整。测定结果为由葡萄糖、甘露糖、葡萄糖醛酸、木糖、岩藻糖组成,其摩尔比为0.24∶1.00∶0.06∶0.29∶0.25。HPLC法对酸性杂多糖组成糖分析是一种比较理想的选择。 相似文献
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本文报道经亲和层析纯化的三齿草藤凝集素(VBL)的糖含量和糖组分的测定结果。经酚-硫酸法测得VBL的总糖含量为4.7%。应用高效液相色谱法对一系列已知标准单糖的定性定量分析条件进行了探索,选用乙腈-水-甲醇=60:30:5体系作流动相,YWG-NH_2作固定相,在高效液相色谱仪中测出VBL含有核糖和鼠李糖,二者摩尔数之比为9.4:1。 相似文献
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氨基酸分析检测方法的研究进展 总被引:2,自引:0,他引:2
对氨基酸分析常用的检测方法:分光光度法、气相色谱法、液相色谱法、毛细管电泳法及其它方法(近红外光谱法、化学发光法、荧光光谱法)进行综述,并介绍了这些方法在氨基酸检测中的应用,为建立快速、高效的氨基酸分析方法提供参考. 相似文献
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《天然产物研究与开发》2016,(11)
利用酶解高效液相色谱法、高效液相色谱法及氯化十六烷基吡啶电位滴定法对鲨鱼硫酸软骨素钠含量进行检测,并对检测结果进行对比分析,结果显示,酶解高效液相色谱法不适用于鲨鱼硫酸软骨素钠含量的测定;而氯化十六烷基吡啶电位滴定法检测鲨鱼硫酸软骨素钠含量稍高于高效液相色谱法;相比之下,高效液相色谱法较适用于检测鲨鱼硫酸软骨素钠含量。 相似文献
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目的:建立测定Beagle犬血浆中灯盏花素浓度的反相高效液相色谱法和液相-质谱联用法,并将其进行多参数的两两比较。方法:采用液-液萃取法处理血清,反相高效液相色谱法测定,流动相为甲醇-水(pH3.0)=42:58,EclipseXDB-C18为固定相;将同样的样品用液相-质谱法开展平行检测;将所测得的数据做两两对比,采用SPSS统计软件进行分析。结果:2种方法测定的数据具有良好的相关性(r=0.982,P〉0.05);最低检测限前者为0.05μg/mL,后者为0.01μg/mL,反相高效液相色谱法的最低检测限和灵敏度不及液相-质谱联用法。结论:反相高效液相色谱法可用于灯盏花素毒代动力学研究,与液相-质谱联用法检测结果无显著差异,且费用较低,不失为-种低成本且行之有效的检测方法。 相似文献
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Summary The compositions of fifty-nine common histological dyes, as well as duplicate samples of several dyes from different suppliers, have been studied by agar gel electrophoresis, agarose gel electrophoresis, paper electrophoresis, paper chromatography and thin layer chromatography. Tables are presented to show the number of components present in each dye as disclosed by the different methods; the cases where duplicate samples were available are summarised in a separate table.On the basis of effectiveness and convenience agar gel electrophoresis and thin layer chromatography were by far the best methods. The Chromatographic method was of slightly wider applicability but as electrophoretic methods gave information on dye charge, agar gel electrophoresis was the best single method. 相似文献
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通过比较4种小鼠粪便细菌总DNA提取方法对基于PCR-DGGE检测的肠道菌群多样性分析的影响,旨在建立适于PCR—DGGE的小鼠肠道微生物宏基因组提取的稳定、经济、快捷的方法。采用SDS裂解法、某国产市售粪便DNA提取试剂盒、改进的化学裂解法、改进的溶菌酶法4种方法提取小鼠粪便细菌总DNA,通过琼脂糖凝胶电泳、紫外分光光度法、细菌16S rRNAV3区PCR扩增结合DGGE对提取结果进行比较分析。SDS裂解法和国产市售试剂盒2种方法提取粪便细菌总DNA均未得到理想结果,另2种方法均能够检测到粪便中20种左右的细菌。改进的化学裂解法和改进的溶菌酶提取法的建立为基于PCR—DGGE进行肠道菌群结构的定量及定性分析提供了可靠的前提基础和实验保障。 相似文献
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Pertti Mörsky 《Analytical biochemistry》1983,128(1):77-85
Factors affecting the activity of human lysozyme (EC 3.2.1.17) toward cell suspensions of Micrococcus lysodeikticus were reexamined. Effects of substrate concentration, pH, and ionic strength and matrix effects of protein were assessed with special emphasis on the interdependence of various parameters. On the basis of these evaluations, an optimized kinetic turbidimetric method for lysozyme assay was set up. The method was applied for automation with a System Olli 3000 analyzer. The new automated lysozyme assay proved good for routine clinical use in regard to analysis speed, sensitivity, linearity, and reproducibility. Reference values for serum, urinary, and cerebrospinal fluid lysozyme were assessed with the automated method. 相似文献
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K. J. Brown 《Applied microbiology and biotechnology》1980,9(1):59-62
Summary A method has been developed for turbidimetric measurement of bacterial growth in standard inexpensive test tubes with closures in-place. Liquid cultures and agar plug diffusion cultures can be assayed using an unmodified spectrophotometer. Growth curves of replicate cultures grown in test tubes, are reproducible with respect to similarity of curve shape, onset of logarithmic growth phase, and maximum growth. 相似文献
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Improved lysis of group N streptococci for isolation and rapid characterization of plasmid deoxyribonucleic acid. 总被引:30,自引:18,他引:12 
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下载免费PDF全文 Procedures for effective cellular lysis and plasmid deoxyribonucleic acid (DNA) isolation from group N streptococci were developed. Cells were grown at 32 degrees C for 4 h in a modified Elliker broth containing 20 mM DL-threonine. After cellular digestion with 2 mg of lysozyme per ml for 7 min at 37 degrees C, 1% sodium dodecyl sulfate exposure resulted in complete and immediate lysis. Lactose (Lac) plasmid species in Streptococcus lactis C2 and S. cremoris B1 (30 and 37 megadaltons, respectively) were demonstrated upon examination of DNA from the cleared lysates by agarose gel electrophoresis. Increasing the lysozyme treatment to 20 min or more resulted in loss of the Lac plasmid, whereas other resident plasmids were unaffected and demonstrable in agarose gels. Diethylpyrocarbonate added before lysis prevented Lac plasmid loss in 20-min lysozyme-treated cells, but was not effective after 40 min of lysozyme treatment. The results suggested that endogenous nuclease activity during the lysozyme treatment period initiated Lac plasmid DNA loss. The development of an efficient lysis procedure for the group N streptococci allowed rapid identification and characterization of plasmid DNA by agarose gel electrophoresis. The plasmid composition of S. lactis C2 and S. cremoris B1, as determined by agarose gel electrophoresis, compared favorably to previous electron microscopic observations. 相似文献
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Improved lysis of group N streptococci for isolation and rapid characterization of plasmid deoxyribonucleic acid. 总被引:31,自引:0,他引:31
Procedures for effective cellular lysis and plasmid deoxyribonucleic acid (DNA) isolation from group N streptococci were developed. Cells were grown at 32 degrees C for 4 h in a modified Elliker broth containing 20 mM DL-threonine. After cellular digestion with 2 mg of lysozyme per ml for 7 min at 37 degrees C, 1% sodium dodecyl sulfate exposure resulted in complete and immediate lysis. Lactose (Lac) plasmid species in Streptococcus lactis C2 and S. cremoris B1 (30 and 37 megadaltons, respectively) were demonstrated upon examination of DNA from the cleared lysates by agarose gel electrophoresis. Increasing the lysozyme treatment to 20 min or more resulted in loss of the Lac plasmid, whereas other resident plasmids were unaffected and demonstrable in agarose gels. Diethylpyrocarbonate added before lysis prevented Lac plasmid loss in 20-min lysozyme-treated cells, but was not effective after 40 min of lysozyme treatment. The results suggested that endogenous nuclease activity during the lysozyme treatment period initiated Lac plasmid DNA loss. The development of an efficient lysis procedure for the group N streptococci allowed rapid identification and characterization of plasmid DNA by agarose gel electrophoresis. The plasmid composition of S. lactis C2 and S. cremoris B1, as determined by agarose gel electrophoresis, compared favorably to previous electron microscopic observations. 相似文献
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Iva Safařik 《Biotechnology Techniques》1991,5(2):111-114
Summary Magnetic biospecific affinity adsorbents for lysozyme isolation have been prepared. They were obtained by incorporation of fine magnetite particles into the structure of chitin, agar or agarose. Hen egg white lysozyme was obtained in 90% purity in one step. 相似文献
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Start Codon Targeted (SCoT) Polymorphism: A Simple,Novel DNA Marker Technique for Generating Gene-Targeted Markers in Plants 总被引:11,自引:0,他引:11
Random amplified polymorphic DNA (RAPD) markers have been used for numerous applications in plant molecular genetics research
despite having disadvantages of poor reproducibility and not generally being associated with gene regions. A novel method
for generating plant DNA markers was developed based on the short conserved region flanking the ATG start codon in plant genes.
This method uses single 18-mer primers in single primer polymerase chain reaction (PCR) and an annealing temperature of 50°C.
PCR amplicons are resolved using standard agarose gel electrophoresis. This method was validated in rice using a genetically
diverse set of genotypes and a backcross population. Reproducibility was evaluated by using duplicate samples and conducting
PCR on different days. Start codon targeted (SCoT) markers were generally reproducible but exceptions indicated that primer
length and annealing temperature are not the sole factors determining reproducibility. SCoT marker PCR amplification profiles
indicated dominant marker like RAPD markers. We propose that this method could be used in conjunction with these markers for
applications such as genetic analysis, bulked segregant analysis, and quantitative trait loci mapping, especially in laboratories
with a preference for agarose gel electrophoresis. 相似文献
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目的 测定铜绿假单胞菌对22种药物的敏感性,帮助临床选择用药。并对分离株进行质粒图谱分析以了解耐药菌株的流行情况。方法 药物敏感性实验采用纸片琼脂扩散法,质粒指纹图谱分析采用碱变性法提取质粒DNA,限制性内切酶切割后进行凝胶电泳分析。结果 铜绿假单胞菌对头胞哌酮、氧派酸、丁胺卡那霉素、壮观霉素、多粘菌毒和头孢三嗪的敏感率在84%-100%之间。所有菌株对其他16种抗性素均有不同程度的耐药。质粒DNA图谱分析显示,12株被检测菌株中有11株含有质粒DNA,其中8株含有23kb质粒DNA。结论 铜绿假单胞菌对头胞哌铜、氟派酸、丁胺卡那霉素、壮观霉素、多粘菌素敏感;多数耐药菌株含23kb质粒DNA。 相似文献
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Possible immunological differences between monkey and human prostate gland proteins and also between seminal vesicle proteins of these species were investigated by agarose gel electrophoresis, agarose gel immunoelectrophoresis and by the agar gel immunodiffusion method, using anti-sera against human plasma, human seminal plasma and human prostatic acid phosphomonoesterase (PMEase). At the same time, the electrophoretic mobility of these prostatic acid PMEases was compared by means of starch gel electrophoresis.Each of these two tissues, monkey and human, was found to contain antigenic proteins with immunological identity. Though antigenic similarity of monkey and human prostatic acid PMEase was demonstrated by immunological methods, a clear difference was observed in the electrophoretic mobility of these enzymes when examined by starch gel electrophoresis. 相似文献