人类泡沫逆转录病毒（Human Spume Retrovirus,HSRV）基因组片段克隆

根据ｐＨＳＲＶ１３全基因组图谱和ｐＢＲＥ３２２质粒载体上限制酶切位点的性质,利用分子克隆技术,使ｐＨＳＲＶ１３质粒上的ｂｅｌ１基因缺失突变并重新构建质粒载体ｐＨＳＲＶ１３－ＢＲ３２２,最后克隆到１株含有目的基因组片段的重组质粒。     

泡沫逆转录病毒Bet蛋白的研究进展

泡沫逆转录病毒能长期感染哺乳动物宿主而不引发疾病,这一特点引起研究者们极大兴趣。有研究发现,泡沫逆转录病毒的辅助蛋白Bet不仅能调控病毒的基因表达和感染周期,对病毒慢性感染的建立有重要作用;还能阻止宿主细胞防御因子APOBEC3对病毒复制产生干扰,与病毒持续性感染的维持有关。为了阐明Bet在病毒复制和感染时所发挥的作用,本文对近年来有关Bet蛋白功能的研究进行了分析和总结。     

复制缺陷型人泡沫逆转录病毒载体构建和外源基因表达

在人泡沫逆转录病毒 (humanfoamyvirus ,HFV)原病毒全长克隆pHRSV13的基础上 ,缺失病毒基因组的env基因和bel基因 ,构建了一个表达标记基因neo和报道基因 gfp的重组人泡沫病毒载体质粒pGPSNI GFP。在与辅助质粒 p△GP共转染情况下 ,得到复制缺陷型的重组病毒颗粒GPSNI GFP。该病毒颗粒可以感染多种宿主细胞 ,将携带的外源基因整合于细胞染色体DNA上并实现表达     

复制缺陷型人泡沫逆转录病毒载体构建和外源基因表达

在人泡沫逆转录病毒(human foamy virus,HFV)原病毒全长克隆pHRSV13的基础上,缺失病毒基因组的env基因和bel基因,构建了一个表达标记基因neo和报道基因gfp的重组人泡沫病毒载体质粒pGPSNI-GFP.在与辅助质粒p△GP共转染情况下,得到复制缺陷型的重组病毒颗粒GPSNI-GFP.该病毒颗粒可以感染多种宿主细胞,将携带的外源基因整合于细胞染色体DNA上并实现表达.     

人类全长功能基因克隆获重大进展

我国科学家参与的人类全长功能基因克隆研究获得重大进展:从4万多个基因中整合出2万多个功能基因,向进一步弄清其确切的功能和结构迈出了一大步,将加快某些疾病的诊断和治疗方法的研究,并对重组蛋白药物的研制有着重要推动作用。这项重大研究由人类基因国际协作研究组完成。科学家对这2万多个整合过的功能基因进行了全面的注释,包括基因组结构、剪接方式、功能结构域、亚细胞定位、代谢途径、基因编码蛋白质的立体结构、基因多态性以及比较基因组分析等。这项成果的重要意义在于:为理解生物学以及在医学、生物技术等方面的应用提供了大量有…     

人类的致病基因

在人类基因组计划取得重大进展的背景下,有1000多种致病基因被克隆鉴定出来并加以分类。定位克隆,定位候选克隆及新兴的SNP标记均被用于搜索新的致病基因。对肿瘤,神经系统和视觉系统等致病遗传基因的研究已获初步成果。     

THF INFLUENCE OF IRRADIANCE ON THF BIOCHEMICAL COMPOSITION OF THE PRYMNESIOPHYTE ISOCHRYSIS SP. (CLONE T-ISO)1

The effects of irradiance on the biochemical composition of the prymnesiophyte microalga, Isochrysis sp. (Parke; clone T-ISO), a popular species for mariculture, were examined. Cultures were grown under a 12:12 h light: dark (L:D) regime at five irradiances ranging from 50 to 1000 μE·m ²·s^?1 and harvested at late-logarithmic phase for analysis of biochemical composition. Gross composition varied aver the range of irradiances. The highest levels of protein were present in cells from cultures grown at 100 and 250 μE·m ³·s¹, and minimum levels of carbohydrate and lipid occurred at 50 μE·m^?2·s^?1. Because the cell dry weight was reduced at lower irradiances, different trends were evident when results were expressed as percentage of dry weights. Protein percentages were highest at Wand 100 μE·m^?2·s^?1 and carbohydrate at 100 μE·m^?2·s^?1. The composition of amino acids did not differ over the range of irradiances. Glutamate and aspartate were always present in high proportions (9.0–13.5%); histidine. methionine, tryptophan, cystine, and hydroxy-proline were minor constituents (0.0–2.6%). Glucose was the predominant sugar in all cultures, ranging from 23.0% (50 μE·m^?2·s^?1) to 45.0% (100 μE·m^?2·s^?1) of total polysaccharide. No correlation was found between the proportion of any of the sugars and irradiance. The proportions of the lipid class components and fatty acids showed little change with irradiance. The main fatty acids were 14:0, 16:0, 16:1(n-7), 18:1(n-9), 18:3(n-3). 18:4(n-3), 18:5(n-3), and 22:6(n-3). Proportions of 22: 6(n-3) increased, whereas l8:3(n-3). 18:3(n-6). and 18:4(n-3) decreased, with increasing irradiance. Pigment concentrations were highest in cultures grown at 50 μE·m^?2·s^?1, except for fucoxanthin and diadinoxanthin (100 μE·m^?2·s^?1). The concentrations of accessory pigments correlated with chlorophyll a, which decreased in concentration with increasing irradiance. On the basts of biochemical composition, an irradiance of 100 μE·m^?1·s^?1 (12:12 h L:D cycle)for the culture of Isochrysis sp. (clone T-ISO) may provide optimal nutritional value for maricultured animals, although feeding trials are now necessary to substantiate this.     

反式激活HIV—1LTR的人疱疹病毒6型（HHV—6）基因片段的初步研究

艾滋病（ＡＩＤＳ）主要是由人免疫缺陷病毒（ＨＩＶ）侵入人体后,破坏人的免疫系统造成的。许多流行病学研究已证明,疱疹病毒与ＨＩＶ的共感染可以导致对ＨＩＶ－１启动子的激活,并加速细胞的病理性反应〔１〕,从而加大个体对ＨＩＶ感染的敏感和加快疾病的进程。人疱...     

OCCURRENCE OF PHYIWATED CHLOROPHYLL c IN ISOCHRYSIS GALBANA AND ISOCHRYSIS SP. (CLONE T-ISO) (PRYMNESIOPHYCEAE)1

The pigment composition of two clones of Isochrysis galbana Parke (CCMP 1323 and CCAP 927/1), and Isochrysis sp. (clone T-ISO) was analyzed by high-performance liquid chromatography using a polymeric octadecylsilica column. Fluorescent peaks with retention times higher than chlorophyll a were detected for all three clones. The corresponding pigments were isolated and characterized in terms of their visible absorbance and fluorescence spectra. The pigments were similar to phytol-substituted chlorophyll c, previously isolated from Emiliania huxleyi (Lohm.) Hay and Mohler and other species containing chlmophyll c₃. The presence of phytol-substituted chlorophyll c in I. galbana which lacked chlorophyll c₃, increases the diversity of chlorophyll patterns for the Haptophyta, which can be grouped, at present, into six different pigment types. This is the jrst observation of a haptophyte containing the apolar phytylated chlorophyll c-like pigment but lacking chlorophyll c₃.     

~(35)S标记探针检测人类单拷贝基因

应用改进的缺口翻译方法,将α-~(35)S-dATP参入DNA分子,获得了>10~8dpm/μgDNA的高比度~(35)S标记探针。用其做Southern吸印杂交探测人类单拷贝基因组织,放射自显影4～10天,能够得到满意的力谱。与~(32)P相比,~(35)S具有半衰期长,无辐射伤害,价格便宜等优点。     

心钠素对卒中易感型自发性高血压大鼠血浆和脑组织加压素的影响

为研究心钠素(ANF)和精氨酸加压素(AVP)的相互作用在原发性高血压发病中的意义,对卒中易感型自发性高血压大鼠(SHRsp)和对照大鼠(WKY)侧脑室(icv)或静脉(iv)注射人ANF-(99-126)观察其对血浆、下丘脑和垂体AVP含量以及平均动脉压(MAP)和尿量(UV)、尿钠(U_(Na)V)排泌的影响。静脉注射ANF后10min,SHRsp和WKY大鼠的MAP分别下降9.4％和12.2％(P<0.05),UV分别增加9和20倍(P<0.01),U_(Na)V增加16和29倍(P<0.01)。侧脑室注射ANF对两种大鼠的MAP、UV和U_(Na)V排泌均无明显作用。静脉或侧脑室注射ANF均使两种大鼠的血浆AVP水平明显下降,其中SHRsp的血浆AVP浓度下降程度(iv,-58％;icv,-31％)弱于WKY大鼠(iv,-80％;icv,-65％),下丘脑AVP含量在两种大鼠中都明显增加,而垂体AVP含量无明显变化。 结果表明,人ANF-(99-126)有明显的抑制AVP释放和降压、利尿、利纳作用,而SHRsp对这些作用的敏感性都降低,提示SHRsp对ABF的反应减弱可能在自发性高血压大鼠的发病中具有一定的意义。     

rDNA片段的序列分析在苦苣苔亚科系统学研究中的应用

本文测定了苦苣苔亚科4族、5属、5种植物的核糖体DNA中的内转录间隔区(ITS)序列及5．8s rRNA基因的3′端序列。这几种苦苣苔亚科植物的ITS-1的长度范围为234～258 bp,ITS-2的长度范 围为218～246bp。Whytockia bijieensis的ITS-1(258bP)和ITS-2(218 bp)在长度、序列及GC含量上 均与其它几个种有较大差异,其代表的尖舌苣苔族可能很早就自苦苣苔亚科的祖先沿单独的一个分支 演化。以w．bijieensis作为功能性外类群,运用PAUP软件分析仅得到一个最简约树。在简约树上, Cyrtandra umbelliferm、Briggsia longipes和Anna mollifolia形成一个单系群,bootstrap分析对该分支的 支持强度达97％,Chirita crasslfolia位于该分支的基部。由于系统树上Cyrtandra umbellifera代表的 浆果苣苔族和Anna mollifolid代表的芒毛苣苔族均起源于长蒴苣苔族,结合这3个族在形态上存在过渡系列,建议将浆果苣苔族和芒毛苣苔族均并入长蒴苣苔族。     

维胺酸对体外转化人支气管上皮细胞及体内构建人支气管上皮组织的抑制作用

癌前改变是肿瘤演变过程中的关键阶段。许多研究显示维甲类化合物对动物肿瘤及体外恶性细胞系具有抑制作用,但尚未见其对肺癌前病变作用的实验室研究报道。人类肺癌的绝大部分起源于支气管上皮,为研究维胺酸对体外转化人支气管上皮M细胞系以及在大鼠气管构建后移植到裸鼠体内生长的具有癌前病变特点的人支气管上皮组织的抑制作用,采用上皮细胞无血清培养技术,人支气管上皮组织大鼠气管内构建／裸鼠皮下移植生长技术,流式细胞学分析,免疫组化、凋亡细胞原位末端标记以及病理学检查等研究方法发现,维胺酸可抑制体外培养的转化人支气管上皮细胞的增殖,使S期细胞比例下降,以及细胞增殖标志Ki-67、mpm-2阳性反应细胞比例下降;明显诱导细胞凋亡。裸鼠腹腔注射给予维胺酸也可使大鼠气管内构建后移植到裸鼠体内生长的癌前期人支气管上皮组织的生长率明显降低,病变程度明显减轻;同样可以诱导细胞凋亡。研究结果提示,维胺酸对体外培养的转化人支气管上皮细胞系及大鼠气管构建／裸鼠体内移植生长的人支气管上皮组织均有明显的抑制作用,是有希望的肺癌化学预防药物。     

酿酒酵母3-磷酸甘油酸激酶基因(PGK1)启动子片段的亚克隆

含有3-磷酸甘油酸激酶基因(PGK1)的酿酒酵母染色体3.1kb HindⅢ片段,已被克隆到大肠杆菌-酵母菌穿梭载体pCN60上。Kpn Ⅰ核酸内切酶在pCN60上没有酶切位点,而在pCN60(PGK1)上仅有一酶切位点。用此酶将pCN60(PGK1)质粒完全酶切,再用Bal31从两端逐步消解碱基对,使反应终止于每端消解500bp左右,加上EcoR Ⅰlinker。用EcoRⅠ、BamH Ⅰ酶切,分离1. 9kb的DNA片段,插入用同样双酶切的酵母启动子探针载体pVC727上,转化E.coli C600,再从转化子中提取重组质粒转化酵母受体菌NA87-11A。用菌落染色法筛选出PHO5基因高效表达转化子,这个转化子质粒含有1.9kb的BamH Ⅰ、EcoRⅠ酶切片段,它具有强启动子功能,并测定其3'末端序列。     

IDENTIFICATION AND CLONING OF AMPLIFIED FRAGMENT LENGTH POLYMORPHISM MARKERS LINKED TO THE MATING TYPE LOCUS OF CHLAMYDOMONAS REINHARDTII (CHLOROPHYTA)

Amplified fragment length polymorphism (AFLP) markers have been widely used to generate molecular maps of plant species, including crops and cereals. We report on a useful protocol to identify AFLPs from Chlamydomonas reinhardtii Dangeard with digoxigenin labeled primers. Although Chlamydomonas has a small genome with a high GC content, we could detect polymorphic bands that led to the identification of several AFLP markers linked to the mating type locus of Chlamydomonas. Three of these markers were isolated from the gel, reamplified, and cloned. The clones were sequenced, and the insertion of the correct fragment was verified in AFLP gels and in Southern blots. One marker showed sequence identity to parts of the fus1 gene, known to be unique in the plus mating type. We also converted some of the AFLP markers into sequence tagged site markers, which allows a fast and convenient screening of progeny of crosses. This procedure will be a useful and fast alternative to the conventional generation of maps for the positional cloning of genes from Chlamydomonas.