关于《微生物学通报》专题刊申请的通知

当前,随着生物技术的飞速发展,微生物学涵盖的领域越来越广,交叉学科的研究也越来越受到关注。除了已有的微生物学、病毒学、基因工程、细胞工程、酶工程、发酵工程之外,基因组学、代谢工程、纳米科学、生物炼制、生物质能等也逐步成为微生物学研究的热门领域。为了更加系统、集中地反映各个领域     

《生物学杂志》征稿简则

1、《生物学杂志》是生命科学的综合性学术期刊,主要刊登动物、植物、微生物及生理、生化、遗传、生物技术、生物工程、分子生物学等生命科学领域的学术论文以及大中专院校生物教学等方面的经验介绍。主要栏目有：研究报告、综述与专论、技术方法、教学研究等。对反映国内外最新研究成果的论文、国家级自然科学基金资助的论文、获省、部级以上资助项目的科研成果论文将优先发表。     

第十一届国际化石刺丝胞与多孔类学术研讨会在比利时召开北大核心CSCD

第十一届国际化石刺丝胞与多孔类学术研讨会于2011年8月21—26日在比利时的列日大学召开。全球27个国家将近有100名代表出席会议。除了东道主比利时外,参加会议的有中国、俄罗斯、美国、英国、法国、加拿大、日本、澳大利亚、德国、意大利、荷兰、爱尔兰、西班牙、瑞士、奥地利、波兰、罗马尼亚、爱沙尼亚、     

关于《微生物学通报》专题刊申请的通知

当前,随着生物技术的飞速发展,微生物学涵盖的领域越来越广,交叉学科的研究也越来越受到关注。除了已有的微生物学、病毒学、基因工程、细胞工程、酶工程、发酵工程之外,基因组学、代谢工程、纳米科学、生物炼制、生物质能等也逐步成为微生物学研究的热门领域。为了更加系统、集中地反映各个领域     

关于《微生物学通报》专题刊申请的通知

当前,随着生物技术的飞速发展,微生物学涵盖的领域越来越广,交叉学科的研究也越来越受到关注。除了已有的微生物学、病毒学、基因工程、细胞工程、酶工程、发酵工程之外,基因组学、代谢工程、纳米科学、生物炼制、生物质能等也逐步成为微生物学研究的热门领域。为了更加系统、集中地反映各个领域     

桑粉虱形态研究

研究描述了容易与杨梅粉虱混淆的重要害虫桑粉虱Pealius mori(Takahashi)成虫、卵、1～4龄若虫及蛹的形状、分类特征,包括成虫的体长、体色、触角、单眼、复眼、口器、翅、足及雌雄外生殖器;卵的形状、大小、卵色及卵柄;1～4龄若虫及蛹的形状、大小、体色、体周的刚毛、触角、口器、足、管状孔、盖瓣、舌状器及腹沟等。并比较桑粉虱与杨梅粉虱的主要分类特征。     

微生物生物技术及其产品的市场浅析

微生物生物技术(或称微生物技术)是一门以应用微生物学为主体的综合性技术群,主要包括微生物学、生物化学、遗传学及基因工程、细胞工程、酶工程、发酵工程和生化工程等。从纵向划分,包括研究、发展和生产。利用微生物技术生产的产品包括酒类、调味品、有机溶剂、有机酸、氨基酸、维生素、抗生素、甾体激素、酶制剂、活性肽及蛋白、酵母及其它单细胞蛋白、淀粉糖等。应用范围包括食品、轻工、医药、农业、化工、矿业和环境保护等方面。     

能排除人体毒素的食物

1．黄瓜：黄瓜原产于印度，又叫青瓜、胡瓜、刺瓜等，其性平、味甘，具有明显的清热解毒、生津止渴等功效。黄瓜中富含蛋白质、糖类、维生素B2、维生素C、维生素E、胡萝卜素、尼克酸、钙、磷、铁等营养成分，同时还含有丙醇二酸、葫芦素、柔软的细纤维等成分，是难得的排毒养颜佳品。     

关于《微生物学通报》专题刊申请的通知

当前,随着生物技术的飞速发展,微生物学涵盖的领域越来越广,交叉学科的研究也越来越受到关注。除了已有的微生物学、病毒学、基因工程、细胞工程、酶工程、发酵工程之外,基因组学、代谢工程、纳米     

关于《微生物学通报》专题刊申请的通知

当前,随着生物技术的飞速发展,微生物学涵盖的领域越来越广,交叉学科的研究也越来越受到关注。除了已有的微生物学、病毒学、基因工程、细胞工程、酶工程、发酵工程之外,基因组学、代谢工程、纳米科学、生物炼制、生物质能等也逐步成为微生物学研究的热门领域。为了更加系统、集中地反映各个领域的研究成果,以及该领域学科的热点难点问题,充分发挥《微生物学通报》的学科引领和导向作用,促进学     

以合成多肽为抗原的戊肝抗体检测试剂的研制

用戊肝病毒（ＨＥＶ）基因组编码氨基酸序列１－９０１－９１４／２－５１５－５３０、３－９１－１２３、２－６１３－６５４相应的三段合成多肽为抗原、研制出一种检测抗－ＨＥＶＩｇＧ的ＥＬＩＳＡ试剂。以该试剂检测中国、缅甸、印度和前苏联肠道传播非乙型肝炎（ＥＴ－ＮＡＮＢＨ）病人血清１０５份,仅３份中国病人血清阴性,阳性率为９７．１％;检查实验感染ＨＥＶＬ赤猩猩血清,感染前阴性,感染后阳性;检查正常人血清９９     

Recognition intensities of submolecular structures,mammalian glyco-structural units,ligand cluster and polyvalency in abrin-a-carbohydrate interactions

Abrin-a is the most toxic fraction of lectins isolated from Abrus precatorius seeds and belongs to the family of type 2 ribosome inactivating proteins (RIP). This toxin may act as a defense molecule in plants against viruses, fungi and insects, where attachment of abrin-a to the exposed glycans on the surface of target cells is the crucial and initial step of its cytotoxicity. Although it has been studied for over four decades, the recognition factors involved in abrin-a-carbohydrate interaction remains to be clarified. In this study, roles of mammalian glyco-structural units, ligand clusters and polyvalency in abrin-a recognition were comprehensively analyzed by enzyme-linked lectinosorbent binding and inhibition assays. The results indicate that: (i) this toxin prefers oligosaccharides having α-anomer of galactose (Gal) at the non-reducing terminal than the corresponding β-anomer; (ii) Galα1-3Galα1- (B_α), Galα1-4Gal (E), Galβ1-3GalNAc (T) and Galβ1-3/4GlcNAc (I/II) related oligosaccharides were the active glyco-structural units; (iii) tri-antennary II_β, prepared from N-glycan of asialo fetuin, played a dominant role in recognition; (iv) many high-density polyvalent I_β/II_β and E_β glycotopes enhanced the reactivity; (v) the carbohydrate recognition domain of abrin-a is proposed to be a combination of a small cavity type of Gal as major site and a groove type of additional one to tetrasaccharides as subsites with a preference of α1-3/4/6Gal, β1-3GalNAc, β1-3/4/6GlcNAc, β1-4/6Glc, β1-3DAra and β1-4Man as subterminal sugars; (vi) size of the carbohydrate recognition domain may be as large enough to accommodate a linear pentasaccharide and complementary to Galα1-3Galβ1-4GlcNAc β1-3Galβ1-4Glc (gailipenta) sequence. A comparison of the recognition factors and combining sites of abrin-a with ricin, another highly toxic lectin, was also performed to further understand the differences in recognition factors between these two type 2 RIPs.     

Macoma birmanica agglutinin recognizes glycoside clusters of β-GlcNAc/Glc and α-Man

Macoma birmanica agglutinin (MBA) that seems to play crucial roles in the innate immunity of marine bivalve, M. birmanica has been earlier defined as GlcNAc/Man specific. However, most complementary carbohydrate structures to its binding domain and ligand clustering in its recognition profile have not been established. In this study, the complete recognition profile of MBA was examined by enzyme-linked lectin-sorbent assay and inhibition assay. Among the monosaccharides tested, GlcNAc was more reactive followed by Man and Glc, others were non-reactive; revealing the importance of equatorial -NAc group at C-2, -OH group at C-4 and C-6, and pyranose conformation of hexose. Moreover, β-glycosides of GlcNAc and Glc were more potent whereas for Man it was α-glycoside. MBA recognized both exposed and internal α-Man and β-GlcNAc/Glc residues well with most linkages except (β1-4). This binding pattern was further extended and confirmed by polyvalent glycoside clusters of GlcNAc(β1-2)Man(α1-, which was a better inhibitor than Man(α1-2/3/6)Man(α1- or Man(α1-3/6)Man(β1- present in well-defined naturally occurring glycoproteins. This broad range specificity explains the importance of MBA as an important pattern recognition molecule that provides more realistic picture of carbohydrate-based immune response triggering.     

Multivalent II [beta-D-Galp-(1-->4)-beta-D-GlcpNAc] and Talpha [beta-D-Galp-(1-->3)-alpha-D-GalpNAc] specific Moraceae family plant lectin from the seeds of Ficus bengalensis fruits

A galactose specific lectin was isolated from the seeds of Ficus bengalensis (Moraceae) fruits and designated as F. bengalensis agglutinin (FBA). The lectin was purified by affinity repulsion chromatography on fetuin-agarose and was a monomer of molecular mass 33kDa. Like other Moraceae family lectins, carbohydrate-binding activity of FBA was independent of any divalent cation. FBA did not bind with simple saccharides, however sugar ligands with aromatic aglycons showed pronounced binding. The combining site of FBA recognized preferably Galbeta1,4GlcNAcbeta1-(II) followed by Galbeta1,3GalNAcalpha1-(Talpha) containing glycotopes. Interaction with saccharides revealed that the combining site of FBA could well accommodate a tetrasaccharide, asialo GM1 glycan (Galbeta1,3GalNAcbeta1,4Galbeta1,4Glcbeta1-), whereas polyvalent Tn (GalNAcalpha1-Ser/Thr), one of the well-recognized ligands of Moraceae family lectin, did not interact well with FBA.     

一种简便高效的改良降落PCR

降落(touchdown,TD)PCR通常涉及15个退火温度,程序设计复杂。报道了一种简便高效的改良降落PCR,只需5个降落退火温度,以杜氏盐藻(Dunaliellabardawil)基因组为模板,设计一对引物扩增胡萝卜素生物合成相关(carotenebiosynthesisrelated,cbr)基因的第3外显子。实验证实该方法程序简单,比标准降落PCR步骤简化70%,且产物的特异性及效率都有较大提高。     

产ESBLs大肠埃希菌和肺炎克雷伯菌呼吸道分离株的基因分型及耐药性分析

目的了解深圳市人民医院大肠埃希菌和肺炎克雷伯菌呼吸道分离株超广谱β-内酰胺酶(ESBLs)的基因型特点及耐药性。方法采用临床实验室标准化协会(CLSI)推荐的表型确证试验筛选出该院呼吸道分离株产ESBLs大肠埃希菌和肺炎克雷伯菌共78株。应用PCR及DNA测序法分析产酶株的TEM、SHV及CTX-M3种β-内酰胺酶基因,用琼脂稀释法测定细菌最低抑菌浓度(MIC)。结果 37株产ESBLs大肠埃希菌中,28株(75.7%)检出CTX-M-14基因,4株(10.8%)检出CTX-M-9基因,其他型较少见。41株肺炎克雷伯菌中,25株(61.0%)检出SHV-12基因,4株(9.8%)检出SHV-11基因,其他SHV型较少。20株(48.8%)检出CTX-M-14基因,5株(12.2%)检出CTX-M-3基因,其他型较少。产ESBL菌株均对亚胺培南敏感,对氨苄西林/舒巴坦的耐药率最高(90%),对其他抗生素有不同程度耐药。结论深圳市人民医院呼吸道分离的产ESBLs大肠埃希菌以CTX-M-14型为主,产酶肺炎克雷伯菌以SHV-12和CTX-M-14型为最常见。     

勒氏笛鲷微卫星位点的筛选及特征分析

采用PCR法快速筛选勒氏笛鲷(Lutjanus russelli)基因组文库, 以获得(CA)_n微卫星位点。勒氏笛鲷基因组DNA经限制性内切酶HaeⅢ+ DraⅠ双酶切后, 连接T-载体克隆, 构建基因组文库。以通用引物M13+/-与重复序列引物(CA)15对基因组文库进行筛选, 二次筛选后得到121个可能含有微卫星位点的阳性克隆。进行序列测定, 共获得53个CA(n≥7)重复序列, 重复次数主要分布于7~15(80.77%)。在所得微卫星序列中, 重复单元除CA外, 还观察到单碱基、三碱基、四碱基、五碱基重复单元。根据侧翼序列设计48对引物, 通过优化PCR反应条件, 可获得清晰可重复的目的条带。研究旨在为勒氏笛鲷遗传多样性研究及遗传图谱的构建等奠定基础, 为勒氏笛鲷资源的合理开发利用提供参考。     

一种简单、快速、高效的基因定点突变方法

小规模抽提含有编码小鼠补体Ⅱ型受体(mCR2)cDNA的质粒,体外合成两对寡核苷酸突变引物,利用PCR反应将突变引入mCR2 cDNA中,即产生P15S和T68Y两种定点突变。然后用DpnI消化PCR产物以去除模板DNA,取适量消化产物转化大肠杆菌XL1-Blue,随机挑选克隆进行测序筛选、鉴定所需突变株。结果表明这一新方法不仅操作简单、快速,而且突变率极高,几乎100％。     

PCR结合反向斑点杂交法检测石蜡包埋组织中的曲霉感染

目的评价PCR结合反向斑点杂交法检测福尔马林固定、石蜡包埋组织中曲霉感染的可行性。方法选取39例病理证实曲霉感染的患者活检标本（21例为鼻窦感染标本、18例为尸检标本）,以1对真菌特有的28SrRNA保守序列结构作为真菌通用引物,以临床常见的4个曲霉菌种：烟曲霉、黄曲霉、黑曲霉、土曲霉的种特异性序列为种特异性探针,与扩增产物进行反向斑点杂交。结果尸检标本阳性率为55．6％（10／18）,鼻窦标本阳性率为76．2％（16／21）,特异性均为100％。在这些曲霉所致的系统性感染中,烟曲霉是主要的致病真菌。结论该方法能对临床无法培养的石蜡组织块进行回顾性病原学研究,并可以鉴定常见的曲霉菌种,有良好的特异性和敏感性,适用于临床曲霉感染的检测。     

赭纤虫RNA聚合酶Ⅰ基因片段的分析

赭纤虫被认为是一类进化过程中较为原始的纤毛虫。本研究以储纤虫基因组DNA为模板,利用锚定PCR技术,扩增出RNA聚合酶I第二大亚基基因片段,并对扩增出的基因片段进行了克隆和序列分析。结果表明：由该基因片段导出的氨基酸序列中共有10个半胱氨酸,均由通用密码子UGU、UGC编码,开放读框中不存在由UGA转译为半眈氨酸这一非通用密码的现象。