用荧光标记O-I噬菌体快速检测食品源沙门氏菌

[目的]利用O-I噬菌体几乎可裂解沙门氏菌属细菌的特性建立快速检测食品中沙门氏菌的方法.[方法]用核酸荧光染料SYBR gold染料标记O-I噬菌体侵染100株试验菌及120份食品样品菌,荧光显微镜鉴定沙门氏菌;并测灵敏度.[结果]100株试验菌中40株沙门氏菌可见杆状荧光,而10株变形杆菌、20株志贺氏菌、20株大肠杆菌和10株葡萄球菌均无荧光;沙门氏菌检测灵敏度达10 CFU/100 μL;120份食品样品中沙门氏菌的O-I噬菌体检测与生化鉴定结果的阳性率分别为9.17%和10%,符合率为91.7%.[结论]试验表明用荧光标记的O-I噬菌体可以快速、直观、准确、大量地检测食品中沙门氏菌.     

Facilitative production of an antimicrobial peptide royalisin and its antibody via an artificial oil-body system

Royalisin found in the royal jelly of Apis mellifera is an antimicrobial peptide (AMP). It has a molecular weight of 5.5 kDa, which contains six cysteine residues. In this study, royalisin was overexpressed in Escherichia coli AD494 (DE3) as two oleosin-fusion proteins for preparation of its antibodies and functional purification. The recombinant royalisin, fused with oleosin central hydrophobic domain in both N- and C-termini, was reconstituted with triacylglycerol and phospholipids to form artificial oil bodies (AOBs). The AOBs were then purified to raise the antibodies. These antibodies could recognize both the native and recombinant royalisins, but not oleosin. Another oleosin-intein S-fusion protein was purified by AOBs system, and royalisin was subsequently released from the AOBs through self-splicing of the intein. The recombinant royalisin exhibited high antibacterial activity, which suggested that it was refolded to its functional structure. These results demonstrated that AOBs system is an efficient method to functionally express and purify small AMPs. In addition, it also provides a facile platform for the production of antibodies against small peptides.     

利用SRAP标记分析中国主栽孔雀草品种的遗传多样性

为了解中国主栽孔雀草品种的遗传背景,采用相关序列扩增多态性(SRAP)分子标记分析了28份孔雀草材料的遗传多样性。14对SRAP引物组合共获得271个位点,其中多态位点151个,占55.72%。每对引物可扩增出14~24条DNA片段,平均19.4条。引物的多态信息含量PIC值在0.693~0.967之间,平均为0.909;每个材料得到的多态性条带比例介于38.78%与51.42%之间,平均46.38%,说明SRAP分子标记可有效鉴别孔雀草种质在分子水平上的遗传变异。品种间的遗传距离值在0.047~0.198之间,平均为0.126;Shannon多样性指数变化于0.178~0.217之间,平均0.201,表明参试的孔雀草材料总体的遗传多样性水平较低。UPGMA聚类后,在遗传距离阈值为0.146处,可将28份材料分为4大类群,与花色表现基本相符,花色可考虑作为孔雀草基于表型分类的主要因子。本研究结果对孔雀草品种鉴定、杂交育种中亲本选配和分子标记辅助选择具有重要意义。     

量子点免疫荧光技术在病理诊断中的初步应用

目的利用量子点(quantum dots,QDs)免疫荧光技术检测石蜡包埋组织中不同蛋白的定位与免疫酶法进行比较,以及两种蛋白的共表达,并探讨其初步应用价值。方法利用QDs免疫荧光和免疫酶组织化学方法分别检测正常阑尾组织LCA、乳腺肌上皮组织Calponin、肺癌组织p53蛋白的表达,并利用QDs免疫荧光双标法同时检测了宫颈上皮内瘤变组织内CK和PCNA蛋白、乳腺癌组织内Her-2和CK蛋白的共表达。结果QDs免疫荧光和免疫酶组织化学技术分别检测LCA、Calponin和p53蛋白的定位完全一致。QDs免疫荧光双标法结合多光谱成像可同时观察到宫颈上皮内瘤变组织内CK和PCNA蛋白、乳腺癌组织内Her-2和CK蛋白的共表达。结论QDs免疫荧光组织化学法具有与免疫酶法等同的应用价值。QDs免疫荧光双标法可同时检测不同蛋白的共定位。     

阿特拉津降解菌ATR3的分离鉴定与土壤修复

阿特拉津因效率高、价格低廉,是我国玉米田施用最广泛的除草剂之一,但其结构稳定,残留时间长,因此对生态环境和人类健康造成了一定的危害。从长期受阿特拉津污染的玉米田土壤中筛选并鉴定阿特拉津降解菌,明确其在不同类型土壤中的去除能力。对分离出的阿特拉津降解菌ATR3进行生理生化分析和16S rRNA序列鉴定,确定菌株ATR3为节杆菌属（Arthrobacter sp.）。该菌株以阿特拉津为唯一氮源,培养48 h后对1 000 mg/L阿特拉津的去除率达到97%以上。敏感作物盆栽试验结果表明,阿特拉津在棕壤上去除最快,褐土次之,黑土最慢,说明阿特拉津在土壤中的去除过程与土壤本身的理化性质呈相关关系。同时,该菌株处理14 d后,能明显恢复玉米的各项生物学指标,说明该菌株对阿特拉津污染土壤具有良好的修复能力。为阿特拉津降解菌剂的推广利用提供参考。     

Rapid isolation and characterization of polymorphic microsatellite loci in the mud crab, Scylla paramamosain (Portunidae)

Scylla paramamosain is a widespread and commercially important species of coastal marine crab. We identified 13 polymorphic microsatellite loci from a genome library constructed with 5'-anchored PCR method. Thirty-two S. paramamosain from the East China Sea were used to analyze the characteristics of these loci. The number of alleles per locus ranged from 3 to 8, with a mean of 5.923. Observed and expected heterozygosities ranged from 0.500 to 0.875 and from 0.500 to 0.859, respectively. Eleven of the 13 loci were highly polymorphic (polymorphic information content >0.5). All of the 13 novel loci were in Hardy-Weinberg equilibrium after Bonferroni's correction (P < 0.0038). There was no null allele, stuttering errors or evidence of allelic dropout in any of the loci analyzed by MICRO-CHECKER. According to pairwise tests, no significant linkage disequilibrium was found among the 13 loci (P < 0.0038, adjusted value). These novel developed microsatellites will be useful for studies of genetic variation, population structure, conservation genetics, and molecular-assisted selective breeding of S. paramamosain.     

外生菌根菌在火炬松人工林应用的研究

连续６年研究了外生菌根菌在火炬松人工林的应用．结果表明,１２个供试菌株均能不同程度地在火炬松根系上形成外生菌根．在１２个供试菌株中,以松林小牛肝菌效果最佳,无论是在苗期还是上山造林,对促进寄主生长的效果均最好,且促进寄主生长的效果在立地条件较差的情况下表现得更为明显．     

Leptin induces insulin-like signaling that antagonizes cAMP elevation by glucagon in hepatocytes

Although many effects of leptin are mediated through the central nervous system, leptin can regulate metabolism through a direct action on peripheral tissues, such as fat and liver. We show here that leptin, at physiological concentrations, acts through an intracellular signaling pathway similar to that activated by insulin in isolated primary rat hepatocytes. This pathway involves stimulation of phosphatidylinositol 3-kinase (PI3K) binding to insulin receptor substrate-1 and insulin receptor substrate-2, activation of PI3K and protein kinase B (AKT), and PI3K-dependent activation of cyclic nucleotide phosphodiesterase 3B, a cAMP-degrading enzyme. One important function of this signaling pathway is to reduce levels of cAMP, because leptin-mediated activation of both protein kinase B and phosphodiesterase 3B is most marked following elevation of cAMP by glucagon, and because leptin suppresses glucagon-induced cAMP elevation in a PI3K-dependent manner. There is little or no expression of the long form leptin receptor in primary rat hepatocytes, and these signaling events are probably mediated through the short forms of the leptin receptor. Thus, leptin, like insulin, induces an intracellular signaling pathway in hepatocytes that culminates in cAMP degradation and an antagonism of the actions of glucagon.     

Preparation of amino-acid-type selective isotope labeling of protein expressed in Pichia pastoris

We report the culture conditions for successful amino-acid-type selective (AATS) isotope labeling of protein expressed in Pichia pastoris (P. pastoris). Rhodostomin (Rho), a six disulfide-bonded protein expressed in P. pastoris with the correct fold, was used to optimize the culture conditions. The concentrations of [alpha-15N] selective amino acid, nonlabeled amino acids, and ammonium chloride, as well as induction time, were optimized to avoid scrambling and to increase the incorporation rate and protein yield. The optimized protocol was successfully applied to produce AATS isotope-labeled Rho. The labeling of [alpha-15N]Cys has a 50% incorporation rate, and all 12 cysteine resonances were observed in HSQC spectrum. The labeling of [alpha-15N]Leu, -Lys, and -Met amino acids has an incorporation rate greater than 65%, and the expected number of resonances in the HSQC spectra were observed. In contrast, the labeling of [alpha-15N]Asp and -Gly amino acids has a low incorporation rate and the scrambling problem. In addition, the culture condition was successfully applied to label dendroaspin (Den), a four disulfide-bonded protein expressed in P. pastoris. Therefore, the described condition should be generally applicable to other proteins produced in the P. pastoris expression system. This is the first report to present a protocol for AATS isotope labeling of protein expressed in P. pastoris for NMR study.