葡萄球菌B型肠毒素突变体的分子设计、高效表达与活性初步研究

葡萄球菌B型肠毒素（SEB0是重要的超抗原,依据SEB分子的晶体结构并结合表面分析,模拟设计了与MHCⅡ类分子和TCR VB区亲合力降低的三位点突变体mSEB(Y89A,C93S,Y94A)。通过PCR重叠延伸法获得突变体基因,导入PBV220载体中,于E.coliDH5α中获得高效表达,纯化的突变毒素T细胞激活活性仅为野生型毒素的1/5左右。     

γ-辐射与常规方法灭活产单核细胞李斯特菌对小鼠免疫原性的比较

【目的】以产单核细胞李斯特菌(Listeria monocytogenes, LM)为模式菌, 比较γ-辐射及常规的热灭活、甲醛灭活制备的灭活李斯特菌对小鼠的免疫原性。【方法】以γ-辐射、热灭活和甲醛灭活法分别制备灭活的LM;腹腔注射BALB/c小鼠,ELISA检测各组灭活菌产生的抗体水平;观察野生型LM攻击后各组的保护效果,动态监测体内带菌情况;流式细胞仪分选免疫小鼠T细胞,以T细胞转移实验评价辐射灭活的LM产生的免疫应答。【结果】 辐射灭活组、热灭活组和甲醛灭活组产生的抗体水平分别为：1:1280, 1:640, 1:160;野生型细菌攻击后这3种灭活菌产生的保护率分别为：100%、35%、30%,其中免疫辐射灭活菌的小鼠能够较快清除攻击的细菌;辐射灭活李斯特菌能够激发产生T细胞保护性免疫应答。【结论】较之传统的灭活方法,利用γ-辐射制备的灭活LM免疫小鼠后能够产生较好的保护效果。     

重组痘苗病毒表达人免疫缺陷病毒中国株B'亚型Gag蛋白及免疫效果观察

为筛选用于我国HIV疫苗的候选基因,利用痘苗病毒载体构建表达HIV-1 B′亚型中国流行株RL42的Gag蛋白的重组病毒rVV-RL42gag,并免疫BALB/c小鼠,检测其诱导的特异性抗体及中和抗体,同时检测其诱导的特异性CTL及与中国流行株C(B′/C重组)亚型和国际流行株A亚型之间的CTL交叉反应.结果显示:重组病毒能很好地表达Gag蛋白,它具有与7株单克隆抗体结合的抗体表位;电镜下可观察到Gag蛋白形成的颗粒.rVV-RL42gag免疫小鼠后能诱导产生高滴度的特异性抗体和CTL,抗体具一定的中和活性,且检测到与C(B′/C重组)亚型和国际流行株A亚型之间的CTL交叉反应.这些结果表明,rVV-RL42gag具有良好的免疫原性,可进一步构建表达HIV B′亚型中国流行株RL42的Gag蛋白的重组痘苗病毒作为候选疫苗.     

免疫A型呼吸道合胞病毒G75-225蛋白的小鼠对病毒感染的抗性

目的:评价A型呼吸道合胞病毒(RSV)G75-225蛋白(G151)与二硫键异构酶(DsbA)的重组蛋白抗原DsbA-G151的免疫活性。方法:采用PCR方法从A型RSVG蛋白扩增G151基因片段,插入表达载体pET-DsbA,经E.coli表达、亲和层析纯化制备DsbA-G151蛋白;将其免疫BALB/c小鼠后获得相应的抗血清,利用ELISA方法、保护性实验检测蛋白免疫活性。结果:构建了表达载体pET-DsbA-G151,表达、纯化获得了重组蛋白DsbA-G151。ELISA检测表明,DsbA-G151能在小鼠体内产生高滴度的特异性IgG;保护性实验显示该蛋白能有效保护BALB/c小鼠不被RSV感染。结论:经ELISA检测、保护性实验,表明DsbA-G151具有良好的免疫原性。     

H9N2禽流感病毒M2 DNA疫苗初免-蛋白加强免疫的保护效果研究

流感病毒M2(基质蛋白2)是A型流感病毒的一个高度保守的蛋白。由于其免疫原性较弱,本研究采用M2 DNA疫苗初免-蛋白加强的策略来考察M2的免疫保护效果。制备A/Chicken/Jiangsu/07/2002(H9N2)流感病毒的M2 DNA疫苗以及经大肠杆菌表达的去除M2跨膜区的M2蛋白即sM2。以SPF级BALB/c小鼠为模型,电击法免疫M2 DNA疫苗,滴鼻法免疫sM2蛋白,免疫间隔三周,并于末次免疫后三周以致死量5LD50流感病毒H9N2攻击小鼠,通过检测小鼠存活率、体重丢失率、肺部病毒滴度及IgG抗体水平等指标来评价免疫的保护效果。实验结果表明,基于M2的疫苗采用DNA疫苗初免蛋白加强免疫二次的免疫程序能诱导较高的特异性抗体,明显减轻小鼠流感病症,提供完全的保护。     

SARS-CoV-2重组S1和S蛋白疫苗诱导保护性免疫的研究*

目的:评价新型冠状病毒(SARS-CoV-2)重组S1蛋白和S蛋白疫苗对SARS-CoV-2的免疫保护效果。方法:将SARS-CoV-2重组S1蛋白和S蛋白分别联合氢氧化铝佐剂以0.1 μg/只、1 μg/只、5 μg/只、10 μg/只不同剂量接种6~8周BALB/c纯系健康雌性小鼠。第二次免疫后采血通过酶联免疫吸附试验(ELISA)检测血清中IgG抗体效价,通过假病毒中和试验比较免疫小鼠血清对SARS-CoV-2野生型株(WT)、英国株(B.1.1.7)、巴西株(P.1)、印度株(B.1.617.2)、Mu毒株(B.1.621)和南非株(501Y.V2-1)六种假病毒毒株中和活性效价,取脾细胞通过酶联免疫斑点技术(ELISpot)检测免疫小鼠的细胞免疫水平。结果:SARS-CoV-2重组S和S1蛋白都能诱导小鼠产生较强的IgG抗体水平。免疫S1蛋白的小鼠血清对SARS-CoV-2野生型株、英国株、巴西株有明显的中和活性,免疫S蛋白的小鼠血清除了对SARS-CoV-2野生型株、英国株、巴西株有明显中和活性之外,对印度株也有明显的中和活性,两种蛋白质免疫的小鼠血清均对野生型株中和效果最强。S蛋白免疫的小鼠脾细胞能够显著诱导出γ干扰素(IFN-γ)和白介素-4(IL-4)的产生。S蛋白诱导产生的IgG抗体、中和抗体、细胞免疫水平均高于S1。结论:SARS-CoV-2重组S蛋白疫苗能够诱导产生较强的保护性免疫应答。     

羧基末端亚单位肽疫苗KLH-Aβ24-42诱导正常BALB/c小鼠制备抗Aβ42抗体

目的:探讨亚单位肽疫苗KLH-Aβ24-42接种小鼠后特异性抗Aβ42抗体的产生情况.方法:将Aβ24-42羧基端与载体蛋白KLH结合制成亚单位肤疫苗免疫BALB/c小鼠.间接ELISA法检测其血清和脑匀浆上清液中的抗体滴度,HE染色对小鼠脑、肝、脾、心、肺和肾行形态学观察抗体毒性.结果:第2次接种后各实验组开始有血清抗体产生,抗体滴度随接种次数的增多而增高;但脑匀浆上清液中未检测到抗体;小鼠各主要脏器均未见病理性变化.结论:亚单位肽疫苗KLH-Aβ24-42越免疫BALB/c小鼠后能产生抗Aβ42抗体,观察未见抗体对各重要脏器的毒性病理.     

柯萨奇病毒A组16型灭活抗原对小鼠免疫保护作用的研究

为了研究柯萨奇病毒A组16型(Coxsackievirus A16,CVA16)灭活抗原在小鼠体内所产生免疫保护作用效果,我们选用CVA16临床分离株521-01T,在Vero细胞中进行大量培养,并对培养产物进行甲醛灭活及超速离心纯化。SDS-PAGE和Western blot对纯化的灭活病毒纯度及性质进行初步分析。Al(OH)3+CVA16及单独CVA16抗原,分别经皮下注射免疫雌性ICR小鼠;相同免疫途径、剂量于第14和28d加强免疫2次。ELISA法检测CVA16特异性血清IgG抗体滴度;微量中和试验法鉴定血清中和抗体滴度;酶联免疫斑点试验(ELISPOT)检测特异性T淋巴细胞的活化。对Al(OH)3+CVA16抗原免疫组母鼠所产仔鼠进行脑腔攻毒,检测母传抗体对新生乳鼠的保护作用。结果显示,Al(OH)3+CVA16灭活抗原在小鼠体内能诱生高滴度的特异性抗体,3次免疫后产生的特异性血清IgG抗体滴度最高可达1∶1×105(P=0.000),中和滴度高于1∶256。同时,该抗原还可以诱导特异性T淋巴细胞的活化。以1 000LD50的病毒量脑腔接种48h内新生乳鼠的病毒攻击实验显示,该母传抗体对新生乳鼠具有100%的保护。这一结果表明该灭活CVA16病毒抗原具有较好的免疫原性及保护性,为CVA16灭活疫苗的研究及评价体系提供了参考。     

羧基末端亚单位肽疫苗KLH—Aβ24-42诱导正常BALB／c小鼠制备抗Aβ42抗体

目的：探讨亚单位肽疫苗KLH—Aβ24-42接种小鼠后特异性抗Aβ42抗体的产生情况。方法：将Aβ24-42羧基端与载体蛋白KLH结合制成亚单位肽疫苗免疫BALB／c小鼠。间接ELISA法检测其血清和脑匀浆上清液中的抗体滴度,HE染色对小鼠脑、肝、脾、心、肺和肾行形态学观察抗体毒性。结果：第2次接种后各实验组开始有血清抗体产生,抗体滴度随接种次数的增多而增高;但脑匀浆上清液中未检测到抗体;小鼠各主要脏器均未见病理性变化。结论：亚单位肽疫苗KLH—Aβ24-42免疫BALB／c小鼠后能产生抗Aβ42抗体,观察未见抗体对各重要脏器的毒性病理。     

单克隆抗体S2C4对2型志贺毒素及其亚型毒性的中和作用

纯化的2型志贺毒素(Shiga toxin 2,Stx2)经福尔马林脱毒后免疫BALB/c小鼠制备Stx2单克隆抗体,用体外中和试验对具有中和活性的阳性抗体克隆进行初筛,对所获得的中和抗体的重、轻链同种型及结合特异性进行鉴定,其中和保护作用通过体内、体外中和试验加以验证,最后,中和抗体对Stx2亚型Stx2c和Stx2vha的中和谱用体内中和试验验证．结果显示,12株抗Stx2的阳性抗体克隆中,只有1株具有中和活性,命名为S2C4,其重、轻链同种型为G₁/κ,其靶分子为Stx2的A亚单位,与Stx2的B亚单位或Stx1不结合．在体外中和试验中S2C4可有效中和Stx2对Vero细胞的杀伤作用,同样,S2C4可中和致死量的Stx2及其亚型Stx2c和Stx2vha对小鼠的毒性作用．该抗体有望成为治疗产志贺毒素大肠杆菌感染的候选分子．     

Modeling of neuropeptide receptors Y1, Y4, Y5, and docking studies with neuropeptide antagonist

Neuropeptide Y (NPY), receptors belong to the G-protein coupled receptor superfamily. NPY mediates several physiological responses, such as blood pressure, food intake, sedation. These actions of NPY are mediated by six receptor subtypes denoted as Y1-Y5 and y6. Modeling of receptor subtypes and binding site identification is an important step in developing new therapeutic agents. We have attempted to model the three NPY receptor types, Y1, Y4, and Y5 using homology modeling and threading methods. The models are consistent with previously reported experimental evidence. To understand the interaction and selectivity of NPY analogues with different neuropeptide receptors, docking studies of two neuropeptide analogues (BVD10 and BVD15) with receptors Y1 and Y4 were carried out. Results of the docking studies indicated that the interaction of ligands BVD10 and BVD15 with Y1 and Y4 receptors are different. These results were evaluated for selectivity of peptide analogues BVD10 and BVD15 towards the receptors.     

神经肽Y及其受体Y1、Y2对痛觉调制的研究进展

神经肽Y（neuropeptide Y,NPY）是一种由36个氨基酸残基组成的肽类激素,属胰多肽家族,广泛分布于中枢及外周神经组织的神经元中。NPY主要参与摄食行为、心血管活动、垂体分泌等生理功能的调节。NPY还参与了痛觉调制。NPY受体有Y1、Y2、Y3、Y4、Y5和Y6六种亚型。目前对Y1受体和Y2受体的研究较多,显示Y1受体和Y2受体参与痛觉调制。但现在对NPY在痛觉中的具体作用机制还不清楚。该文对NPY及其Y1受体、Y2受体在痛觉调制中的作用作一概述。     

Characterization of Yersinia enterocolitica, Y. intermedia, Y. aldovae, Y. frederiksenii, Y. kristensenii and Y. pseudotuberculosis by electrophoretic polymorphism of acid phosphatase, esterases, and glutamate and malate dehydrogenases

Acid phosphatase, esterases, and glutamate and malate dehydrogenases of 192 strains of Yersinia enterocolitica, Y. intermedia, Y. aldovae, Y. frederiksenii, Y. kristensenii and Y. pseudotuberculosis were analysed by horizontal polyacrylamide agarose gel electrophoresis and by isoelectrofocusing in thin-layer polyacrylamide gels. The six species were clearly separated from each other by their distinct enzyme electrophoretic polymorphism. For Y. enterocolitica, the strains of biotype 5 were differentiated from the other biotypes by the mobility of glutamate dehydrogenase. For Y. frederiksenii, six zymotypes were delineated by pI and by the mobility of the enzymes. Variation in number or mobility of esterases within each species could represent a marker for epidemiological and ecological analyses. A linear relationship was obtained between the mean genetic diversity coefficient of enzymes and the mean percentage DNA-DNA relatedness of Y. intermedia, Y. aldovae, Y. enterocolitica and Y. frederiksenii.     

Yersiniae other than Y. enterocolitica, Y. pseudotuberculosis, and Y. pestis: the ignored species

The genus Yersinia is composed of 11 species, of which three (Y. pestis, Y. pseudotuberculosis, and Y. enterocolitica) have been exhaustively characterized. The remaining eight species (Y. frederiksenii, Y. intermedia, Y. kristensenii, Y. bercovieri, Y. mollaretii, Y. rohdei, Y. ruckeri, and Y. aldovae) have not been studied extensively and, because of the absence of classical Yersinia virulence markers, are generally considered to be nonpathogenic. However, recent data suggest that some of these eight species may cause disease by virtue of their having virulence factors distinct from those of Y. enterocolitica. These data raise intriguing questions about the mechanisms by which these species interact with their host cells and elicit human disease.     

A neuropeptide Y receptor Y1-subfamily gene from an agnathan, the European river lamprey. A potential ancestral gene.

We report here the isolation and functional expression of a neuropeptide Y (NPY) receptor from the river lamprey, Lampetra fluviatilis. The receptor displays approximately 50% amino-acid sequence identity to all previously cloned Y1-subfamily receptors including Y1, Y4, and y6 and the teleost subtypes Ya, Yb and Yc. Phylogenetic analyses point to a closer relationship with Y4 and Ya/b/c suggesting that the lamprey receptor could possibly represent a pro-orthologue of some or all of those gnathostome receptors. Our results support the notion that the Y1 subfamily increased in number by genome or large-scale chromosome duplications, one of which may have taken place prior to the divergence of lampreys and gnathostomes whereas the second duplication probably occurred in the gnathostome lineage after this split. Functional expression of the lamprey receptor in a cell line facilitated specific binding of the three endogenous lamprey peptides NPY, peptide YY and peptide MY with picomolar affinities. Binding studies with a large panel of NPY analogues revealed indiscriminate binding properties similar to those of another nonselective Y1-subfamily receptor, zebrafish Ya. RT-PCR detected receptor mRNA in the central nervous system as well as in several peripheral organs suggesting diverse functions. This lamprey receptor is evolutionarily the most distant NPY receptor that clearly belongs to the Y1 subfamily as defined in mammals, which shows that subtypes Y2 and Y5 arose even earlier in evolution.     

A Y2 receptor mimetic aptamer directed against neuropeptide Y.

Neuropeptide Y (NPY) is a 36-amino acid neuropeptide that exerts its activity by at least five different receptor subtypes that belong to the family of G-protein-coupled receptors. We isolated an aptamer directed against NPY from a nuclease-resistant RNA library. Mapping experiments with N-terminally, C-terminally, and centrally truncated analogues of NPY revealed that the aptamer recognizes the C terminus of NPY. Individual replacement of the four arginine residues at positions 19, 25, 33, and 35 by l-alanine showed that arginine 33 is essential for binding. The aptamer does not recognize pancreatic polypeptide, a highly homologous Y4 receptor-specific peptide of the gut. Furthermore, the affinity of the aptamer to the Y5 receptor-selective agonist [Ala(31),Aib(32)]NPY and the Y1/Y5 receptor-binding peptide [Leu(31),Pro(34)]NPY was considerably reduced, whereas Y2 receptor-specific NPY mutants were bound well by the aptamer. Accordingly, the NPY epitope was recognized by the Y2 receptor, and the aptamer was highly similar. This Y2 receptor mimicking effect was further confirmed by competition binding studies. Whereas the aptamer competed with the Y2 receptor for binding of [(3)H]NPY with high affinity, a low affinity displacement of [(3)H]NPY was observed at the Y1 and the Y5 receptors. Consequently, competition at the Y2 receptor occurred with a considerably lower K(i) value compared with the Y1 and Y5 receptors. These results indicate that the aptamer mimics the binding of NPY to the Y2 receptor more closely than to the Y1 and Y5 receptors.     

A satellited Y chromosome]

A previous report in 1967 on the observation of a satellited Y chromosome found in a French Canadian family line is confirmed by the use of the ammoniacal silver procedure which stains selectively the nucleolus organizer regions (NORs) in acrocentric human chromosomes. There is evidence that this peculiar chromosome results from the translocation to the distal end of the Y chromosome long arms of a satellited segment from a D or G autosome.     

A mosaic XY1Y2/XY1Y2Y2 common shrewSorex araneus

XY₁Y₂/XY₁Y₂Y₂ mosaicism was found in a wild adult common shrewSorex araneus (Linnaeus, 1758) in lymphocytes from spleen. The multiple sex chromosome system in the common shrew was the result of an X-autosome translocation and the Y₂ chromosome was the unpaired autosome present in males. The external phenotype of the shrew was that of a mormal male. The histological picture of its testis showed complete spermatogenic breakdown on the stage of primary spermatocytes, hence the shrew was sterile. The possible causes of spermatogenic arrest in a mosaic shrew are dis cussed.     

Natural antimicrobial susceptibilities and biochemical profiles of Yersinia enterocolitica-like strains: Y. frederiksenii, Y. intermedia, Y. kristensenii and Y. rohdei

The natural susceptibility of 131 Yersinia strains of Y. frederiksenii (n=38), Y. intermedia (n=48), Y. kristensenii (n=26) and Y. rohdei (n=19) to 70 antibiotics was tested. Minimum inhibitory concentration (MIC) values were determined with a microdilution procedure in IsoSensitest broth (all strains) and cation-adjusted Mueller Hinton broth (some strains). All species were naturally sensitive or sensitive and of intermediate susceptibility to tetracyclines, aminoglycosides, acylureidopenicillins, numerous cephalosporins, carbapenems, aztreonam, quinolones, chloramphenicol, folate-pathway inhibitors, nitrofurantoin, and fosfomycin. Uniform natural resistance was found with penicillin G, oxacillin, several macrolides, lincosamides, streptogramins, glycopeptides, rifampicin and fusidic acid. Species-specific differences in susceptibility affecting clinical assessment criteria were seen with aminopenicillins (in the presence and absence of beta-lactamase inhibitors), ticarcillin and some cephalosporins. Major medium-dependent susceptibilities were found with fosfomycin. beta-Lactam MIC susceptibility patterns suggested that most strains of the species tested produce both class A and class C (AmpC) beta-lactamases that are characteristic for the species. The present study describes a database concerning the natural susceptibility of some Y. enterocolitica-like species to a wide range of antibiotics, which can be applied to validate forthcoming antibiotic susceptibility tests of these strains and might contribute to their identification. An evaluation of 30 biochemical tests that secured phenotypic identification to the Yersinia species level is presented.