非洲猪瘟病毒特点及扬州大学对其研究简介

非洲猪瘟是目前威胁世界养猪业最危险的传染病,强毒感染猪致死率高达100%。该病在沙哈拉以南28个非洲国家呈地方性流行,2007年传入格鲁吉亚后很快传播到10多个临国,目前在高加索地区和俄罗斯广泛流行,我国沈阳也有首例报道。非洲猪瘟病毒具有许多独特特点,目前无安全有效的疫苗,一旦发生必须实行严格的隔离封锁、猪群销毁和感染场地消毒,对社会、经济造成巨大的影响,因此快速、准确诊断十分重要。扬州大学孙怀昌教授带领的团队对非洲猪瘟分子诊断进行了深入研究,为我国非洲猪瘟防控提供了系统的技术与试剂储备。

大鼠腰椎腹侧神经根牵拉模型的建立

目的为了研究肌萎缩侧索硬化症致病机理和药物研发,建立第4腰椎腹侧神经根牵拉大鼠模型,并用脑源性神经营养因子作为阳性药物进行模型的有效性验证。方法首先对5只SD雄性大鼠进行手术,一周后用抗胆碱乙酰转移酶抗体进行免疫组织化学染色观察脊髓前角运动神经元数量的变化;预实验证明手术模型成功后,将40只7周龄SD雄性大鼠随机分为四组,两组模型对照组及两个脑源性神经营养因子治疗组(手术后立刻预防性给药组和手术后一周治疗性给药组)。使用抗胆碱乙酰转移酶免疫组织化学染色观察运动神经元数量的变化。结果大鼠手术后恢复良好,临床观察无异常。染色结果证明手术牵拉后,造成明显的脊髓前角运动神经元变性死亡。与对照组相比,用脑源性神经营养因子治疗的神经根牵拉动物,不管是预防性给药还是手术1周后再进行治疗性给药都达到了良好的治疗效果,胆碱乙酰转移酶染色阳性神经元细胞数量显著增加(P<0.0001),结果分别为17.85%比93.06%;26.6%比87.27%。结论成功的建立大鼠第4腰椎腹侧神经根牵拉模型,为肌萎缩侧索硬化症的研究提供了一种有价值的动物模型。

联合注射牛γ干扰素和人溶菌酶表达质粒对奶牛乳房炎的治疗效果

通过乳腺注射牛γ干扰素（BoINF-γ）和人溶菌酶（LYZ）表达质粒,比较单独和联合注射重组质粒与抗生素对奶牛乳房炎的治疗效果。将PCR扩增的BoINF-γc DNA插入真核表达载体pcDNAK,用重组质粒pcDNAK-BoINF-γ转染NIH 3T3细胞,经免疫荧光试验证明,重组质粒能正确表达。将91个奶牛乳房炎乳区分为4组,通过乳腺穿刺法注射,第1组注射400μg pcDNAKLYZ,第2组注射400μg pcDNAK-BoINF-γ,第3组注射400μg pcDNAKLYZ和400μg pcDNAK-BoINF-γ,第4组注射100 IU青霉素和25μg链霉素,次日重复注射1次。在注射后10 d进行临床症状观察、乳汁体细胞检测和细菌培养计数。结果显示：注射pcDNAKLYZ对临床型乳房炎的治疗效果为80%,对隐性乳房炎的治疗效果为79.2%;注射pcDNAK-BoINF-γ对临床型乳房炎的治疗效果为50%,对隐性乳房炎的治疗效果为66.7%;联合注射pcDNAKLYZ和pcDNAKBoINF-γ对临床型乳房炎的治疗效果为100%,对隐性乳房炎的治疗效果为83.5%;青链霉素合剂对临床型乳房炎的治疗效果为50%,对隐性乳房炎的治疗效果为60%。试验结果表明,联合注射人溶菌酶和牛γ干扰素表达质粒对奶牛乳房炎具有更好的治疗效果。

Efficient generation of transgenic chickens using the spermatogonial stem cells in vivo and ex vivo transfection

The highly efficient novel methods to produce transgenic chickens were established by directly in-jecting the recombinant plasmid containing green fluorescent protein (GFP) gene into the cock's testis termed as testis-medianted gene transfer (TMGT), and transplanting transfected spermatogonial stem cells (TTSSCs). For the TMGT approach,four dosages of pEGFP-N1 DNA/cationic polymer complex were injected intratesticularly. The results showed: (1) 48 h after the injection,the percentages of testis cells expressing GFP were 4.0%, 8.7%, 10.2% and 13.6% in the 50, 100, 150 and 200 μg/mL group, re-spectively. The difference from the four dosage groups was significant (P<0.05). On day 25 after the injection, a dosage-dependent and time-dependent increase in the number of transgenic sperm was observed. The percentages of gene expression reached the summit and became stable from day 70 to 160, being 12.7%, 12.8%, 15.9% and 19.1%, respectively. The difference from the four dosage groups was also significant (P<0.05). (2) 70 d after the injection, strong green fluorescent could be observed in the seminiferous tubules by whole-mount in-situ hybridization. (3) 70 d after the injection, the semen was collected and used to artificially inseminate wild-type females. The blastoderms of F1 and F2 transgenic chicken expressed GFP were 56.2% (254/452) and 53.2% (275/517), respectively. The detec-tion of polymerase chain reaction (PCR) of F1 and F2 transgenic chicken blood genomic DNA showed that 56.5% (3/23) of F1 and 52.9% (9/17) of F2 were positive. Southern blot showed GFP DNA was in-serted in their genomic DNAs. (4) Frozen whole mount tissue sections of F1 and F2 transgenic chicken liver, heart, kidney and muscle showed that the rates of green fluorescent positive were between 50.0% and 66.7%. (5) With the TTSSCs method, SSCs ex vivo transfected with GFP were transplanted into recipient roosters whose endogenic SSCs had been resoluted. The donor SSCs settled and GFP ex-pression became readily detectable in the frozen whole mount tissue sections of recepient testes. Moreover, sperms carrying GFP could be produced normally. The results of artificially inseminating wild-type females with these sperms showed 12.5% (8/64) of offspring embryo expressed GFP and 11.1% (2/18) hatched chicks were tested transgenic. Our data therefore suggest TMGT and TTSSCs are the feasible methods for the generation of transgenic chickens.