唐菖蒲球茎芽的离体培养及快速繁殖

将带1-2个芽眼的唐菖蒲球茎切块接种到附加1.0mg/LBA的MS基本培养基上可诱导休眠芽萌动、无菌芽转移至附加3.0mg/LBA的培养基上可分化产生丛生芽。丛生芽的继代增殖宜采用附加1.5mg/LBA的培养基生根培养,以MS+NAA 0.1-0.5mg/L或MS+IBA 1.5mg/L效果最佳。试管苗移栽存活率可达50%左右。     

Distribution of rDNA loci in the genus Glycine Willd.

The objective of this study was to examine the distribution of rDNA loci in the genus Glycine Willd. by fluorescent in situ hybridization (FISH) using the internal transcribed spacer (ITS) region of nuclear ribosomal DNA as a probe. The hybridized rDNA probe produced two distinct yellow signals on reddish chromosomes representing two NORs in 16 diploid (2n=40) species. Aneudiploid (2n=38) and aneutetraploid (2n=78) Glycine tomentella Hayata also exhibited two rDNA sites. However, the probe hybridized with four chromosomes as evidenced by four signals in two diploid species (Glycine curvata Tind. and Glycine cyrtoloba Tind.) and tetraploid (2n=80) G. tabacina (Labill.) Benth. and G. tomentella. Synthesized amphiploids (2n=80) of Glycine canescens F. J. Herm. (2n=40) and the 40-chromosome G. tomentella also showed four signals. This study demonstrates that the distribution of the rDNA gene in the 16 Glycine species studied is highly conserved and that silence of the rDNA locus may be attributed to amphiplasty during diploidization and speciation. Received: 10 October 2000 / Accepted: 6 December 2000     

慢性蜜蜂麻痹病病毒核酸与蛋白质组分的研究

从自然感染的意大利麻痹病蜂(APis mellifera)头部,经二次差速离心与蔗糖梯度离心获得纯化的慢性蜜蜂麻痹病病毒(CBPV)。纯化的CBPV制备物感染正常蜜蜂,4天后出现典型的麻痹症状,接着死亡,平均死亡率分别为95％与100％。SDS-聚丙烯酰胺凝胶电泳分析,二次差速离心初步纯化的病毒制备物含有多条蛋白带,而蔗糖密度梯度纯化的病毒制备物仅含有单一的多肽带。5％、7.5％与10％SDS-聚丙烯酰胺凝胶电泳分析,均检测出一种病毒蛋白质,分子量大约为24,200道尔顿,而且不同凝胶浓度检测的蛋白质分子量相近。慢性蜜蜂麻痹病病毒核酸也用SDS-聚丙烯酰胺凝胶电泳分析,结果表明,凝胶中有5条带,对核酸酶敏感,证明该病毒含有5个单股RNA组分。对慢性蜜蜂麻痹病病毒的基因组结构进行了讨论。     

Quantitative polymerase chain reaction as a reliable method to determine functional lentiviral titer after ex vivo gene transfer in human mesenchymal stem cells

BACKGROUND: Human mesenchymal stem cells (hMSCs) are a promising target for ex vivo gene therapy and lentiviruses are excellent gene transfer vehicles in hMSCs since they achieve high transduction rates with long-term gene expression. Nevertheless, senescence of hMSCs may limit therapeutic applications due to time-consuming cell selection and viral titration. Here, we describe a fast and reliable method to determine functional lentiviral titer by quantitative polymerase chain reaction (qPCR) after highly efficient ex vivo gene transfer in hMSCs. METHODS: Lentivirus production was tested with different types of packaging systems. Using p24 ELISA remaining viral particles were detected in the cell culture supernatant. The lentiviral gene transfer efficiency was quantified by FACS analysis. Lentiviral titers were determined by qPCR of expressed transgenes. RESULTS: Third-generation self-inactivating vectors showed highly efficient gene transfer in hMSCs. No viral antigen was detected in the cell culture supernatant after four media changes, suggesting the absence of infectious particles after 4 days. We observed a linear correlation between virus dilution and level of transgene expression by qPCR analysis, therefore allowing viral titering by quantification of transgene expression. Finally, we demonstrated that transduced hMSCs retained their stem cell character by differentiation towards adipogenic, osteogenic and chondrogenic lineages. CONCLUSIONS: Quantification of transgene copy numbers by qPCR is a fast and reliable method to determine functional lentiviral titer after ex vivo gene transfer in hMSCs.     

从cDNA文库中筛选分析阳性克隆的简便方法

cDNA文库中阳性克隆的传统筛选分析法既费时又费力.利用微波炉加热的方法,简化了原位杂交中噬菌斑裂解、DNA变性与固定的程序;进一步运用PCR扩增技术,特异扩增克隆载体中插入的cDNA片段,加快了阳性克隆分析的进程.     

表达人高致病性禽流感病毒H5N1(安徽株)结构基因的DNA疫苗在小鼠中诱导的免疫应答分析

本研究旨在研发经济、高效的人高致病性禽流感病毒H5N1实验疫苗并优化免疫方案。首先优化并合成H5N1(安徽株)的血凝素基因(HAop)和神经氨酸酶基因(NAop)并证实其正确表达,再构建含有H5N1(安徽株)结构基因的多个单顺反子(HAwt、HAop和NAop)和双顺反子(HAop/M2和NAop/M1)DNA疫苗质粒。随后,采用不同途径的体内电转法在第0周和第3周2次免疫Balb/C小鼠,初步分析了抗原特异性体液免疫(HA血凝抑制抗体,NA特异性抗体,中和抗体)和细胞免疫应答(IFN-γELISpot)的特点。结果表明:含有优化血凝素基因(HAop)和优化神经氨酸酶基因(NAop)的DNA疫苗可以快速激发较强的免疫应答,尤其是细胞免疫应答;皮内电转所激发的体液免疫应答强于肌肉电转。本研究为新型H5N1疫苗的研发以及免疫方案的优化奠定了基础。     

虎纹蛙促性腺激素释放激素分泌调节的离体研究

利用离体静态孵育系统和放射免疫测定法,研究了性成熟的虎纹蛙雌蛙离体的视前－下丘脑－正中隆起（P－H－ME）片段促性腺激素释放激素（GnRH)的分泌调节。结果表明：γ－氨基丁酸（GABA）对成熟前期蛙离体P－H－ME片段的哺乳类GnRH（mGnRH)的释放有显著的刺激作用;随着GABA作用浓度的增加,刺激作用逐渐增强。100μmol/L的多巴胺（DA）及1μmol/L和10μmol/L的雌二醇(E2）则显著抑制鸡ⅡGnRH(cGnRH-Ⅱ)的释放。10μmol/L和100μmol/L的睾酮（T）以及10μmol/L的E2显著刺激冬眠期蛙P－H－ME片段mGnRH的释放。这些结果表明,GABA,DA及E2和T对虎蚊蛙GnRH的释放有直接的调节作用。     

缓/控释肥料研究进展

缓/控释肥料对作物产量的影响因作物种类、肥料种类和试验条件而异,大多数植物增产比较明显,如大豆使用长效尿素,与普通尿素相比增产幅度最高可达33%。各种类型的缓/控释肥料,均可不同程度的提高肥料利用率。缓/控释肥料在农业上的应用能有效地保护生态环境,如抑制土壤NH4 向NO3-氧化,减少土壤NO3-的积累,从而减少氮肥以NO3-形式淋溶损失,减少了施肥对环境的污染;可以减少土壤N2O的释放等。提出了目前缓/控释肥料在农业应用中存在的问题及今后的发展方向。     

细菌核糖体的结构和功能

二十多年来,国际上几家实验室独立地竞争性地应用高分辨率X-射线衍射技术在原子水平上绘制出了细菌完整核糖体及其亚基精细的三维结构图,为其生物功能的研究提供了清晰的结构基础。由于这项伟大的科学成果,美国科学家文卡特拉曼·拉马克里希南（Venkatraman Ramakrishnan）、托马斯．施泰茨（Thomas A．Steitz）和以色列女科学家阿达．约纳特（Ada E．Yonath）三人荣获2009年度诺贝尔化学奖。细菌核糖体是细胞中合成蛋白质的一种细胞器,包括大小不同的两个亚基,由3种RNA和50多种不同的蛋白质组成。     

基质金属蛋白酶-2/9敏感型可跨膜融合抗氧化酶的表达、纯化和表征北大核心CSCD

融合了跨膜肽的抗氧化酶可进入细胞,保护细胞免受放射损伤。然而跨膜肽的跨膜能力没有靶向性,其也可把抗氧化酶带入肿瘤细胞进而保护肿瘤细胞,降低放疗的效果。为此,根据多数肿瘤细胞微环境中存在活性基质金属蛋白酶(matrix metalloproteinase,MMP)-2或MMP-9的特点,在细胞跨膜肽R9与人铜、锌超氧化物歧化酶(superoxide dismutase 1,SOD1)和谷胱甘肽S-转移酶(glutathione S-transferase,GST)之间融合MMP-2/9的底物肽X,设计了融合蛋白GST-SOD1-X-R9。该蛋白在肿瘤微环境中可因MMP-2/9酶切底物肽X而失去跨膜肽,从而无法进入肿瘤细胞,进而只能进入正常细胞。全基因合成SOD1-X-R9序列,并将其插入原核表达载体pGEX-4T-1中,得到表达质粒,并实现了GST-SOD1-X-R9融合蛋白的可溶表达。GST-SOD1-X-R9经硫酸铵沉淀和GST亲和层析纯化,分子量约为47 kDa,与理论值一致。纯化的融合蛋白的SOD活性和GST活性分别为2954 U/mg和328 U/mg。GST-SOD1-X-R9的SOD活性或GST活性在生理条件下几乎没有变化。该融合蛋白在溶液中可被胶原酶Ⅳ部分水解。分别建立了2D和3D培养的HepG2细胞模型来检验肿瘤微环境中的MMP-2活力对该蛋白跨膜能力的影响。在2D培养模型中,HepG2的MMP-2活力极低,但在3D培养模型中,随着培养时间的增加,HepG2肿瘤球的体积变大,其胞外MMP-2活力也随之增强。GST-SOD1-X-R9在2D培养的HepG2细胞中具有和GST-SOD1-R9蛋白一样的跨膜效率,但在3D培养的HepG2细胞球中的跨膜能力大大降低。本研究为后续深入研究GST-SOD1-X-R9靶向防护正常细胞的氧化损伤效应奠定了基础。