中华蜜蜂蜂毒磷脂酶A_2基因在大肠杆菌中的表达(英文)

将中华蜜蜂蜂毒磷脂酶A2(AcPLA2)蛋白成熟肽编码区基因(405 bp)克隆至表达载体pETBlue-1,在大肠杆菌Tuner(DE3)plac I中诱导表达,经SDS-PAGE电泳检测,表达产物分子量为15kD,约占细菌总蛋白的4.6％;用意大利蜜蜂蜂毒磷脂酶A2(AmPLA2)纯品制备的兔源多克隆抗体为一抗作Western blot,表达产物显示类似于天然纯AmPLA2的特异性印迹,证实AcPLA2基因已在大肠杆菌中得到表达。     

中华蜜蜂工蜂王浆腺活性的变化

本试验以短期体外放射化学测定法,测定了中华蜜蜂(Apis cerana cerana)工蜂的王浆腺(HP)的活性,以意大利蜂(Apis mellifera ligustica)进行对比.结果表明工蜂的HP在体外培养液中1—6小时掺入的放射性DPM几乎呈直线增加.春夏繁殖期,中华蜜蜂7日龄工蜂的HP活性最强,而意大利蜜蜂是10日龄.中华蜜蜂的越冬工蜂的HP虽呈发育状态,但活性低.而在早春,当蜂群内部出现幼虫时,越冬工蜂的HP又呈现活性.     

中蜂处女王性成熟日龄及其交尾习性的探讨

本研究对210只人工培育的出房后1,2,3,4,6,8．10日龄的中蜂处女王受精囊液的pH值进行测定．结果表明,1日龄处女王受精囊液的pH值平均为7．7,2日龄为8．5,从3日龄开始达到最高值8.8．并保持稳定状态,由此判断出房后3日龄的中蜂处女王性已成熟．通过对72只中蜂处女王交尾飞行的观察,结果表明,蜂王交尾日龄多为6-8日．最早为4日龄,最迟为16日龄;处女王认巢飞行持续时间平均为7．4分钟,交尾飞行平均为21．5分钟：处女王连续交尾飞行1-3次,有9只处女王在一天里进行2次交尾飞行．     

EXPRESSION OF A BEE-VENOM PHOSPHOLIPASE A2 FROM APIS CERANA CERANA IN ESCHERICHIA COLI

Abstract  The venomous phospholipase A₂ (AcPLA₂) coding reading region of the Chinese honeybee ( Apis cerana cerana ), which is composed of 405 bp encoding a mature glycosylated peptide with 134 amino residues was transformed into the expression vector pETblue-1. Then the recombinant vector was introduced into Escherichia coli Tuner (DE3) plac I for expression. Analysis result of SDS-PAGE showed that the expression products had a protein band of about 15kD. Detection of western blot using ant-European honeybee ( Apis mellifera ) phospholipase A₂ (AmPLA₂) polyclonal serum as the first antibody showed that the expression products appeared a special blot same as the native AmPLA₂.The result demonstrated that the AcPLA₂ peptide had been expressed in E. coli and the AcPLA₂ has the similar antigenicity as the AmPLA₂.     

CLONING AND SEQUENCING OF GENE ENCODING HYALURONIDASE FROM THE VENOM OF APIS CERANA CERANA*

Abstract The venomous hyaluronidase (Hya) gene of Chinese honey bee, Apis cerana cerana, was amplified by RT‐PCR from total RNA of venom glands of the worker bees. The full length of its nucleotide is 1164 bp encoding a 387 amino acid polypeptide with predicted molecular weight of 42.6 kD. The alignment of AcHya amino acid sequence with other 6 Hyas shows that AcHya is most closely related to the Hya of European honey bee, A. mellifera, with 91% amino acid identity. It also shares homology with Hya of Dolichovespul amacidata, Polistes annularis, Vespula vulgaris, Lutzomia longipalpis and Homo sapiens (sperm), with 54%., 52%., 46%, 27% and 20% amino acid identity, respectively. A phylogenetic tree of those hyaluronidases was drawn by using GENETYX program, the conservation, the relationship between molecular structure and function of 7 hyaluronidases as above was compared and analysed.     

中华蜜蜂蜂毒透明质酶基因的克隆与序列分析(英文)

从中华蜜蜂工蜂毒腺中快速抽提总RNA ,用RT PCR方法扩增得到该蜂毒的透明质酸酶 (AcHya)基因 ,其核苷酸序列全长为 1 1 6 4bp ,可编码 3 87个氨基酸残基 ,预计分子量为 42 .6kD。将所推导出的氨基酸序列与其它 6种透明质酸酶 (Hya)氨基酸序列比较 ,结果表明 ,AcHya与意大利蜜蜂Hya非常相似 ,具有91 %的同源性 ,与长黄胡蜂Hya、常见黄胡蜂Hya、、马蜂Hya、吸血沙蠓唾腺Hya、人精液PH2 0Hya的同源性分别为 5 4 %、5 2 %、46 %、2 7%和 2 0 %。同时根据氨基酸序列用GENETYX程序绘制了 7种Hya的分子系统树 ,并根据同源性比较分析了 7种Hya的保守性、结构与功能的关系     

中华蜜蜂磷酸甘油变位酶（PhosphoglycerateMutase）基因的序列分析

在中华蜜蜂(Apis cerana)工蜂毒腺cDNA库内发现了一个插有1104bp外源片段的克隆,内含一个765bp的开放阅读框架(ORF),编码一个含有254．个氨基酸残基的依赖于2,3一二磷酸甘油酸的磷酸甘油变位酶(dPGAM),催化3一磷酸甘油和2一磷酸甘油之间的转化。推测的氨基酸序列与其他7种生物的dPGAM的相似性很高(39％-88％),而与其他4种不依赖于2,3-二磷酸甘油酸的磷酸甘油变位酶(iPGAM)的相似性则很低(10％-12％),氨基酸序列的多重联配表明组成dPGAM活性位点的氨基酸残基在包括中华蜜蜂在内的所有生物体内是十分保守的,Ac—PGAM是一种典型的dPGAM。这是昆虫纲中继在果蝇中发现PGAM基因后的第2个昆虫dPGAM基因,其对PGAM基因的结构与功能研究及对昆虫的分子生物学研究具有意义。同时,对PGAM的进化关系的分析表明该基因可以用作研究物种系统关系的一个依据。     

中国东方蜜蜂不同地理种群的RAPD分析

本研究采用RAPD技术对来自中国境内8个省市的28群东方蜜蜂Apis cerana进行了研究,探讨了它们之间的亲缘关系.结果表明:15条随机引物共扩增产生了155条谱带,其中单个弓l物扩增的谱带数为4～16条,多态性条带为122条,多态比率为78.7%;不同种群东方蜜蜂遗传多样性丰富,遗传距离变化较大,最大为0.4197(海南-北京),最小为0.0933(江西-甘肃);聚类结果显示8个地理种群的东方蜜蜂可聚为3个聚类簇,且各地理种群的亲缘关系与空间距离正相关.     

SEQUENCE ANALYSIS OF A NOVEL INSECT PHOSPHOGLYCERATE MUTASE GENE FROM THE CHINESE HONEYBEE,APIS CERANA*

A clone inserted with 1 104 bp fragment containing a 765bp Open Reading Frame(ORF), encoding a putative 2,3‐bisphosphoglycerate(2,3BPG) dependent Phosphoglycerate mutase(dPGAM) that catalyzes the transfer of a phosphate group from the C3 carbon atom to the C2 carbon atom of phosphoglycerate, was screened by mass sequencing from the cDNA library of the venom glands of Apis cerana. The deduced amino acid sequence shared high similarities (39% ‐ 88%)with the dPGAM of 7 other organisms, but the similarities with the iPGAM of 4 other organisms were low (10% ‐ 12%). Moreover, the alignment of Ac‐PGAM with the dPGAMs from 7 other organisms showed that all the active site amino acid residues were conserved. This result shows that Ac‐PGAM is a typical dPGAM. Thus, this is the second PGAM gene reported in Insecta. Furthermore, phylogenetic analysis showed that the evolutionary tree of PGAMs reflects the systematic relationship of species.     

意蜂和中蜂四种同工酶的研究

用聚丙烯酰胺凝胶等电聚焦电泳分析了意蜂和中蜂的酯酶(Est)、异柠檬酸脱氢酶(Idh)、苹果酸酶(Me)和苹果酸脱氢酶(Mdh)同工酶.两个蜂种的四种同工酶谱有不同程度的差别、意蜂酯酶Ⅳ和苹果酸脱氢酶Ⅲ是多态性的;中蜂的四种同工酶没有多态现象.     

中华蜜蜂工蜂蜡腺细胞的超微结构

本文描述了中华蜜蜂(Apis cerana)成体工蜂蜡腺细胞的超微结构.通过电镜观察发现蜡腺细胞具有许多质膜内陷形成的管腔,作为蜂蜡或其前体物的输送通道.细胞质中富含线粒体及粗面内质网,细胞核为不规则的形状,细胞质中还含有少量溶酶体,微管和微丝等结构.     

中华蜜蜂咽下腺的电镜观察

王浆是由工蜂的咽下腺所分泌,咽下腺位于工蜂头腔内两侧,每侧腺体都有一条长而粗的分泌管,在分泌管的两侧平行排列有许多椭圆形小叶,每个小叶内有十多个细胞,每个细胞有一根胞外管与分泌管直接相通,细胞内有一条胞内管又与胞外管相连。王浆就是通过细胞内分泌块分泌而成,由胞内管把王浆输送到胞外管,最后由分泌管到咽喉部,在此处饲喂王浆给蜂王、幼蜂和雄蜂。通过咽下腺的超微结构观察,不仅了解到咽下腺各种细胞器的形态特征,同时也了解到输送王浆的途径。     

中华蜜蜂工蜂触角感受器的扫描电镜观察

对中华蜜蜂(Apis cerana)工蜂触角感受器的扫描电镜观察,见到在触角上有九种类型的感受器,它们是板形感器、腔锥感器、坛形感器、钟形感器、锥形感器、毛形感器A、毛形感器B、毛形感器C和D、缘感器以及各种类型的刚毛等.对于这些感受器的外部形态和分布部位进行了详细地观察和描述,发现中华蜜蜂与西方意蜂(Apis mellifera)有差异.     

感染囊幼病的工蜂咽下腺细胞的超微结构的变化

前言 中华蜜蜂囊幼病是我国养蜂业的一种重要病毒病,发病率很高,有的地区造成大量的幼虫死亡,给我国养蜂生产带来一定的危害,为了对防治病害提供科学的依据,我们首先对该病病原进行了分离、提纯及电子显微镜的研究等工作。发现该病毒对幼虫和成蜂,尤其对工蜂体内各个器官都有程度不同的影响。在幼虫发病期症状特别明显,病幼虫身体松软多水,其表皮容易破裂,当悬挂幼虫时其幼虫末端积聚有透明的液滴,在巢房内幼虫头部尖并变成黑色,头部稍微向上抬起呈船形。死后的幼虫干涸变为褐色的外壳留于巢房内,当感染的幼虫全部封盖后,巢房盖的中央有一小孔,这些异常的变化都是囊幼病的典型症状。幼虫症状虽很明显,但工蜂感染病毒后在外部形态上却没有明显     

A homozygous female hemophilia A

BACKGROUND:

Hemophilia A (HA), being an X-linked recessive disorder, females are rarely affected, although they can be carriers.

AIMS:

To study the mutation in F8 gene in an extended family with a homozygous female HA.

MATERIALS AND METHODS:

All the seven affected members (six males and one female) were initially screened by Conformation Sensitive Gel Electrophoresis (CSGE) and direct DNA sequencing.

RESULTS:

A homozygous missense mutation c.1315G>A (p.Gly420Ser) was identified in exon 9 of F8 gene in homozygous state in the affected female born of 1° consanguinous marriage and in all the affected male members of the family. Her factor VIII levels was found to be 5.5%, vWF:Ag 120%.

CONCLUSION:

In India, as consanguineous marriages are very common in certain communities (up to 30%), the likelihood of encountering female hemophilia is higher, although this is the first case of HA out of 1600 hemophilia families registered in our Comprehensive Haemophilia Care Center. Genetic diagnosis in such cases is not necessary as all the male children will be affected and daughters obligatory carriers.     

Aminopeptidase A is angiotensinase A

Summary Quantitative histochemical measurements of aminopeptidase A (APA; E.C.3.4.11.7) were done kinetically in the kidney glomeruli of rat and mouse with an instrumental setup consisting of a microdensitometer and a computer-supported morphometric system. The histochemical demonstration of APA was carried out using the simultaneous azo coupling technique (purest-grade Fast Blue B as coupling agent and -l-glutamic acid-4-methoxy-2-naphthylamide as substrate). The methodological studies show that APA activity is calcium-ion-dependent and increases linearly with the thickness of the tissue section (3–12 m) and that the time-course of APA activity as determined by linear regression is linear only for the first 1 to 2 min of the reaction. — Kinetic measurements indicate a 40% decrease in APA activities when -l-glutamic acid-4-methoxy-2-naphthylamide (-l-Glu-MNA) is replaced by -l-aspartic acid-4-methoxy-2-naphthylamide. When -l-Glu-MNA is replaced with l-alanine-4-methoxy-2-naphthylamide, which is a substrate of aminopeptidase M (APM) only very low reaction rates are measurable (about 1.4% of those with -l-Glu-MNA). 100 and 130 mM NaCl in the incubation medium increase APA activities by approximately 16%–17%. — To clarify the functional importance of APA in the kidney, their activities were measured under the influence of angiotensins. The glomerulus was selected as the measuring site, for besides APA it contains no APM or other peptidases that could degrade angiotensins (the glomerular dipeptidyl peptidase IV is not inhibited by angiotensin II). Using the Lineweaver-Burk plot, we determined a K _m of 0.16 mM for the APA in rat glomeruli and 0.14 mM in mouse glomeruli. The V _max in mouse glomeruli is 1.6 times higher than in rat glomeruli. Ang iotensin I, II and III competitively inhibit APA in the rat and mouse glomeruli. — With quantitative histochemical techniques it was possible to show that APA is equivalent to angiotensinase A (splitting off the N-terminal aspartic acid from angiotensin I and II).Supported by the Deutsche Forschungsgemeinschaft (SFB 105)     

A glucoside of urospermal A

The aerial parts of Urospermum picroides afforded, in addition to urospermal A a p-hydroxylphenyl acetate of a glucoside of urospermal A.