血链球菌拮抗可疑牙周病原菌机理探讨Ⅱ细菌素的产生及影响因素

血链球菌产生细菌素（血链素）至培养上清液中，无论是需氧或厌氧环境，血链球菌均可产生血链素。采用无水乙醇沉淀法提取血链球菌培养上清液中的蛋白质，运用ＳＤＳ－ＰＡＧＥ分析其蛋白成份，发现有１３０ｋｄ、１２０ｋｄ、７４ｋｄ、和５６ｋｄ四条蛋白区带，通过电泳凝胶弥散法抑菌试验显示，５６ｋｄ蛋白带具很强的抑菌活性，提示此蛋白质可能为血链素的所在位置。     

血链球菌拮抗可疑牙周病原菌机理探讨：Ⅱ细胞素的产生及…

血链球菌产生细菌素至培养上清液中,无论是需氧或厌氧环境,血链球菌均可产生血逻素。采用无水乙醇沉淀法提取血链球菌培养上清液中的蛋白质,运用ＳＤＳ－ＰＡＥＧ分析其蛋白成份,发现１３０ｋｄ、１２０ｋｄ、７４ｋｄ、和５６ｋｄ四条蛋白区带,通过电泳凝胶弥散法抑菌试验显示,５６ｋｄ蛋白带具很强的抑菌活性,提示此蛋白质可能为血链素的所在位置。     

一株抗真菌内生多粘芽孢杆菌的分离鉴定及对水稻恶苗病菌的抑制作用

目的：从番茄叶片中筛选具广谱抑真菌活性的拮抗内生细菌,研究其对水稻恶苗病菌的抑制作用。方法：采用对峙培养法筛选拮抗内生细菌,根据菌株形态、生理生化特性结合16S rRNA基因序列分析鉴定菌株;采用硫酸铵沉淀法提取抗菌粗蛋白,研究其对水稻恶苗病菌菌丝生长和孢子萌发的影响。结果：从番茄叶片中筛选到一株抗真菌内生多粘芽孢杆菌（Paenibacillus polymyxa）SD-6,该菌株具有广谱抑菌活性,对供试的13种植物病原真菌均具较强的抑制作用;该菌株产生的抗菌粗蛋白能够显著抑制水稻恶苗病菌菌丝生长和孢子萌发,并能导致萌发孢子畸形和破裂。结论：从番茄叶片中分离到一株能产生抗真菌蛋白并具有广谱高效抑真菌作用的内生多粘芽孢杆菌,该菌株及其抗菌蛋白具有防治水稻恶苗病的潜力。     

八种中草药抑菌试验报告

笔者采用药物平板稀释法对常州地区八种中草药进行抑菌试验,并测定其ＭＩＣ（最低抑菌浓度）,结果显示：一年蓬、小飞蓬、三叶鬼针草、朝天委陵菜、艹律草、羊蹄等有较强抑菌作用,提示可作为对革兰阳性菌和革兰阴性菌的抗菌中草药。     

一种兔肠源抗菌蛋白分离纯化及其抑菌活性

目的探讨兔肠道组织抗菌有效成分的组成及其性质。方法将新鲜兔小肠组织匀浆,经高温处理,乙酸浸提后,检测抗菌活性,再经Sephadex G100和Sephadex G75凝胶柱过滤层析,收集具有抗菌活性的蛋白组分,经SDS-PAGE电泳,考马斯亮蓝染色后,为一条蛋白带,其相对分子质量约为43×103。用琼脂糖弥散法和活菌计数实验检测纯化物对9株细菌的抑菌作用。结果分离得到一种纯的兔肠源抗菌蛋白,纯化的兔肠源抗菌蛋白对9株细菌的均有明显的抑菌作用,杀菌率介于78%与98%之间,显示了较强的抗菌活性。结论初步显示了兔肠源抗菌蛋白在细菌性疫病的防治方面的应用前景。     

生殖道中具有抑菌活性乳酸菌的分离筛选及其抑菌物质分析

目的 从阴道炎患者的棉拭子样本中分离筛选具有抗菌活性乳酸菌,为研究对细菌性阴道炎具有确实疗效的微生态制剂提供理论与菌种保证.方法 应用纯培养技术及双层平板法从阴道样品中分离筛选具有较好抑菌活性的乳酸菌.通过有机酸排除试验、过氧化氢排除试验和蛋白类抑菌物质排除试验对具有较好抑菌活性菌株的主要抑菌物质分析,并通过PCR反应对是否具有细菌素相关基因进行鉴定.结果 从7个棉拭子样本中共分离得到26株乳酸菌,其中有6株呈现抑菌活性.K4M2、K4M5、K4M6和K4M8菌株的主要抗菌物质为有机酸.而K4M9、K4M10两株植物乳杆菌的主要抗菌物质除有机酸外,尚可以产生细菌素.病原菌拮抗试验结果表明,这两株菌株的混合培养上清对具有较好的抑菌效果.结论 K4M9、K4M10菌株有望作为微生态制剂用于细菌性阴道炎的临床防治.     

小羽贯众提取物抗菌活性的初步研究

目的：比较小羽贯众根状茎和叶提取物体外抑菌活性。方法：牛津杯法和96孔板法,通过测定抑菌圈大小、最小抑菌浓度（MIC）和最小杀菌浓度（MBC）,比较小羽贯众根状茎和叶提取物分别对10种常见细菌的抑制作用,以及不同产地抑菌效果的比较。结果：小羽贯众的根状茎和叶的提取物对10种常见的细菌均表现出较强的抑菌活性,肺炎克雷伯氏菌对提取物最敏感。结论：小羽贯众提取物作为一种天然的抗菌物质,具有广谱抗菌效果,有较高的应用潜力和开发前景。     

左肾动脉缩窄诱导心肌肥大大鼠心肌蛋白差异表达研究

目的：应用蛋白质组学方法分析病理性心肌肥大心肌细胞蛋白表达特征。方法：雄性SD大鼠16只,分为2组（n=8）：两肾一夹组（2K1C）和假手术组（SO）,术后饲养8周,使用普通多普勒和组织多普勒鉴定动物模型,然后提取心肌总蛋白,应用二维凝胶电泳技术,建立分辨率高和重复性良好的凝胶图像,质谱（MALDI—TOF-MS）鉴定差异蛋白点,与网络数据库进行匹配,并对鉴定蛋白进行分类。结果：两肾一夹大鼠心肌细胞有21个蛋白点表现出显著增加或减少,经数据库匹配,获得14种差异表达的蛋白质。结论：两肾一夹大鼠心肌出现一些差异表达蛋白席官们可能在病理性心肌肥大的发生中起重要作用。     

贪婪倔海绵中抗菌活性细菌的筛选及初步鉴定

采用平板涂布法从我国南海三亚周边海域贪婪倔海绵（Dysidea avara）中分离海绵共附生细菌,采用金黄色葡萄球菌、大肠埃希氏菌、荧光假单胞菌、枯草芽孢杆菌、白假丝酵母、宛氏拟青霉、黑曲霉7种指标菌进行抑菌试验筛选抗菌活性菌,同时对于得到的活性菌进行生理生化鉴定。共分离获得个149个细菌菌株,发现20株具有抑制真菌和革兰氏阳性细菌的活性,占细菌总数的13．4％。经过细菌形态观察和生理生化试验,发现此20株活性菌属于革兰氏阳性芽孢杆菌属（Bacillus sp．）。     

Biolog细菌自动鉴定系统应用初探

利用BiloogMicrostation细菌自动鉴定系统（3.50版）对已知的9个属23株菌进行了鉴定。24hBiolog系统鉴定结果：12林革兰氏阴性菌中,9株可准确鉴定到种的水平（75％）,3株未达到属的水平。11株革兰氏阳性菌均属于芽孢杆菌属,全部鉴定到属的水平,9株准确鉴定到种的水平（81.8％）。总计属的水平准确率86.9％（20／23）,种的水平准确率78.2％（18／23）。     

单细胞凝胶电泳技术及在土壤生态毒理学中的应用

单细胞凝胶电泳技术又称为彗星实验,是最近几年发展起来的一种快速、简单、灵敏、可靠的检测细胞核DNA损伤的技术。总结了近几年来单细胞凝胶电泳技术的发展、原理、方法及其应用,并指出其下一步的发展趋势。彗星实验中,镶嵌于琼脂糖中的细胞核在电场中向正极移动,因细胞核与DNA片段迁移速率不同,而形成类似“彗星”的图像。目前采用的彗星实验有多种,可以检测诸如DNA双链断裂、单链断裂、碱不稳定位点等多种类型的DNA损伤。碱性彗星实验因其高灵敏度而被广泛采用。彗星实验的主要步骤包括细胞核悬浮液的获得、彗星电泳胶板制备、细胞裂解、DNA变性解旋、电泳、中和、染色和观察等。目前彗星实验广泛应用于各个研究领域,近年来开始用于环境污染的基因毒性研究和生物监测,并取得了迅速发展。     

Influence of growth media on vancomycin resistance of Enterococcus isolates and correlation with resistance gene determinants

The effect of Mueller-Hinton (MH), MH+blood or brain heart infusion medium (agar or broth) on 13 Enterococcus isolates was determined, when testing their antibiotic susceptibility. Disk diffusion and Vitek methods were used to determine vancomycin resistance, while broth dilution and E-test methods were used to measure the minimum inhibitory concentration. The data were correlated with the presence of vancomycin resistance genes. A definite correlation pattern could not be established between the presence of van genes and vancomycin resistance in any plating medium, when tested by the disk diffusion assay. The broth dilution, irrespective of the plating medium, and Vitek methods were more reliable than the E-test method in testing isolates with vanA or vanB genes. However, for vanC2/C3 genotypes, the E-test method, irrespective of the plating medium, tested better than the broth dilution assay.     

Comparison of various culture methods (Skirrow medium, a blood-free medium and a filtration system enriched in Bolton and Preston broths) for isolation of Campylobacter spp. from raw meat samples

We compared six procedures and investigated the optimal method for isolation of Campylobacter spp. from raw meat samples. Ninety-nine meat samples were enriched in Bolton broth and Preston broth, followed by plating on Skirrow, mCCDA, and blood agar (a membrane filter on its surface) media, respectively. Thirty-nine of 99 samples were positive and 71 Campylobacter were isolated by one or more methods. More than one species of Campylobacter were obtained in 8 (20.5 %) of 39 positive samples and two genotypes were yielded on the same medium (11 samples, 28.2 %) by pulsed-field gel electrophoresis (PFGE) genotyping. Enrichment by Preston broth was significantly better than by Bolton broth (P?<?0.05). Moreover, the latter failed to detect Campylobacter jejuni strains. Skirrow medium was significantly less efficient than mCCDA medium and membrane filtration method (P?<?0.05). Overall, the combination of PC (primary enrichment in Preston broth, followed by selective enrichment on mCCDA agar), PF (primary enrichment in Preston broth, followed by membrane filtration culture onto blood agar), and BF (primary enrichment in Bolton broth, followed by membrane filtration culture onto blood agar) methods provided the optimum isolation rate of Campylobacter spp.     

A sensitive standardised micro-gel well diffusion assay for the determination of antimicrobial activity

We have developed a highly sensitive micro-gel well diffusion assay for the determination of antimicrobial activity. In essence, the normal radial diffusion type assay was adapted to perform it in a microtiter plate. We compared our micro-gel well diffusion assay to a radial diffusion assay and a microtiter broth dilution method, using gramicidin S as model antibiotic, and Micrococcus luteus as the indicator organism. The micro-gel well diffusion assay was as sensitive as the microtiter broth dilution method, and approximately twice as sensitive as the radial diffusion method. Data analysis to calculate minimum inhibitory concentration, 50% microbial growth inhibition and maximum inhibitory concentration was refined by generating dose-response curves with the software package Prism 3.0 (Graphpad Software Inc.). The minimum inhibitory concentrations, determined by the three methods, were significantly different (P<0. 001), highlighting the limitations involved in comparing data obtained from different methods.     

一种高效快速的鱼类标本基因组DNA提取方法

以95%酒精保存的黄鳝(M onopterus albus)和斑鳢(Channa maculates)标本为材料,采用先沉降DNA再去除杂质的方法从鱼类标本中提取基因组DNA。基因组DNA的琼脂糖凝胶电泳和紫外分光光度法检测以及PCR扩增结果显示,本方法提取的鱼类基因组DNA的电泳主带清晰明亮;A260/A280值在1.7830-2.0144之间;PCR扩增产物条带清晰明亮,且单一整齐没有拖带,表明本方法可从酒精保存的鱼类标本中提取比较纯净的DNA,能够满足一般分子生物学试验需要。与传统苯酚/氯仿法相比,本方法操作简单快速,避免了苯酚等物质对后续实验的影响,可作为一种常规动物组织DNA提取方法。     

一种简便快速筛选重组子的方法

目的：根据碱裂解法抽提质粒DNA的原理,研究应用快检缓冲液方法挑取重组子克隆,从而获得简单易行,快速方便,节省时间,提高工作效率的筛选重组子的方法。方法：不需抽提质粒,只要将菌落接入快检缓冲液后直接进行普通琼脂凝胶电泳分析,就可以快速筛选出重组子。结果：结果和提取质粒酶切鉴定结果一致。结论：经实验证明用快检缓冲液方法筛选重组子是一种简单易行,快速方便,节省时间,提高工作效率并且可靠的方法。     

Loop-mediated isothermal amplification (LAMP) for rapid detection of Renibacterium salmoninarum, the causative agent of bacterial kidney disease

A loop-mediated isothermal amplification (LAMP) assay was developed for rapid, specific and sensitive detection of Renibacterium salmoninarum in 1 h without thermal cycling. A fragment of R. salmoninarum p57 gene was amplified at 63 degrees C in the presence of Bst polymerase and a specially designed primer mixture. The specificity of the BKD-LAMP assay was demonstrated by the absence of any cross reaction with other bacterial strains, followed by restriction digestion of the amplified products. Detections of BKD-LAMP amplicons by visual inspection, agrose gel electrophoresis, and real-time monitoring using a turbidimeter were equivalently sensitive. The BKD-LAMP assay has the sensitivity of the nested PCR method, and 10 times the sensitivity of one-round PCR assay. The lower detection limit of BKD-LAMP and nested PCR is 1 pg genomic R. salmoninarum DNA, compared to 10 pg genomic R. salmoninarum DNA for one-round PCR assay. In comparison to other available diagnostic methods, the BKD-LAMP assay is rapid, simple, sensitive, specific, and cost effective with a high potential for field application.     

Comparison of selective media for assay of coliphages in sewage effluent and lake water.

Selective media, including EC medium, gram-negative broth, nutrient broth (with 0.05% sodium deoxycholate), and lactose broth (with 0.05% sodium deoxycholate), as well as nonselective nutrient and lactose broths, were compared for the enumeration of coliphages by the agar layer method from activated-sludge effluent and eutrophic-lake water from a lake receiving treated sewage effluent. Samples were plated directly or after chloroform treatment with Escherichia coli B, E. coli C, or a mixed host of both E. coli B and C. With the exception of gram-negative broth, direct assays of all samples with the selective media generally resulted in significantly higher (P less than 0.05) recoveries of coliphages than did assays of chloroform-treated samples with nutrient broth medium regardless of the host used. In addition, chloroform pretreatment resulted in decreased recovery of coliphages with each selective medium in most analyses. The highest recoveries of coliphages from all samples with each host, except lake water with E. coli C, were obtained by direct assay on EC medium. The selectivity of the EC and gram-negative media resulted in suppression of bacterial interference on direct assay plates comparable to that observed in nutrient agar medium with chloroform-treated samples. The use of certain selective media for the direct assay of environmental materials for coliphage may enhance the recovery of coliphages and obviate bacterial decontamination procedures.     

Comparison of selective media for assay of coliphages in sewage effluent and lake water

Selective media, including EC medium, gram-negative broth, nutrient broth (with 0.05% sodium deoxycholate), and lactose broth (with 0.05% sodium deoxycholate), as well as nonselective nutrient and lactose broths, were compared for the enumeration of coliphages by the agar layer method from activated-sludge effluent and eutrophic-lake water from a lake receiving treated sewage effluent. Samples were plated directly or after chloroform treatment with Escherichia coli B, E. coli C, or a mixed host of both E. coli B and C. With the exception of gram-negative broth, direct assays of all samples with the selective media generally resulted in significantly higher (P less than 0.05) recoveries of coliphages than did assays of chloroform-treated samples with nutrient broth medium regardless of the host used. In addition, chloroform pretreatment resulted in decreased recovery of coliphages with each selective medium in most analyses. The highest recoveries of coliphages from all samples with each host, except lake water with E. coli C, were obtained by direct assay on EC medium. The selectivity of the EC and gram-negative media resulted in suppression of bacterial interference on direct assay plates comparable to that observed in nutrient agar medium with chloroform-treated samples. The use of certain selective media for the direct assay of environmental materials for coliphage may enhance the recovery of coliphages and obviate bacterial decontamination procedures.