异羟基洋地黄毒甙元(Digoxigenin)标记的探针在乙型肝炎病毒核酸杂交中的应用

应用异羟基洋地黄毒甙元标记的探针,检测了人和鸭的血清及肝脏中的乙型肝炎病毒核酸,并与~(32)P标记的同位素探针做了比较。结果证明,该探针的特异性和敏感性与同位素探针一致(0.2pg)。它可用于各种核酸杂交试验,如打点杂交、Southern和Northern转印杂交试验等。恰当地从标本中提取待测核酸,是应用该探针的重要条件。     

地高辛配基标记核酸技术及其应用

核酸探针通过地高辛配基(异羟基洋地黄毒苷配基)标记的脱氧尿嘧啶核苷三磷酸(Dig-dUTP)随机引物插入结合而被标记,然后辅以免疫酶化学检测等新技术。和放射性同位素标记探针一样,它已广泛用于核酸等物的各种探测及分析,具有灵敏、安全、简便、经济及实用等优点。     

豌豆间期细胞核内核仁组织者区排列的非放射性原位杂交定位

以异羟基洋地黄毒甙（ｄｉｇｏｘｉｇｅｎｉｎ）ｓｆｉ ｙｎ ｒ ｒＲＮＡ为探针与多聚甲醛固定的植物根振动切片原位杂交。结合免疫荧光检测分析了豌豆（Ｐｉｓｕｍ ｓａｔｉｖｕｍ）间期细胞核内核仁组织者区的数目、分布和排列。研究结果发现豌豆根尖分生组织间期细胞核内有１－６个被探针分子强烈标记的位点。这些位点呈大小不等（０．２４－１．９８μｍ＾３）的斑点状,分布在核仁的周边,并且与核仁相连。探针标记位点在核     

豌豆间期细胞核内核仁组织者区排列的非放射性原位杂交定位

以异羟基洋地黄毒甙(digoxigenin)标记的rRNA为探针与多聚甲醛固定的植物根尖振动切片原位杂交。结合免疫荧光检测分析了豌豆(Pisum sativum)间期细胞核内核仁组织者区的数目、分布和排列。研究结果发现豌豆根尖分生组织间期细胞核内有1—6个被探针分子强烈标记的位点。这些位点呈大小不等(0.24-1.98μm~3)的斑点状,分布在核仁的周边,并且与核仁相连。探针标记位点在核仁周边的排列方式随标记位点的数目不同而异。在具有四个标记位点的细胞核内,它们呈四面体,梯形或平行四边形排列。在显示原位杂交阳性的细胞核中,59.5%显示4个标记位点,少于或多于4个标记位点的细胞分别占35.7%和4.76%。探针标记位点的数目与标记位点本身的大小无明显联系,而与核仁的体积大体上呈负相关趋势。文章讨论了这些被rRNA探针标记的位点与核仁组织区及核仁形成的关系。     

性腺甾体激素对雌,雄大鼠下丘脑血管升压素mRNA水平的影响

实验用１０－１１周龄经阉割的雌、雄Ｓｐｒａｇｕｅ－Ｄａｗｌｅｙ大鼠进行。以３末端异羟基洋地黄毒甙标记的２６个碱基长的寡核苷酸作为检测探针,用核酸斑点杂交技术检测大鼠下丘脑血管升压素ｍＲＮＡ水平。在假手术对照组,雄性大鼠下丘脑ＡＶＰｍＲＮＡ水平经雌性大鼠高４５％（Ｐ〈０．０５）,血浆渗透压高于雌性大鼠（Ｐ〈０．０５）。摘除卵巢的大鼠下丘脑ＡＶＰｍＲＮＡ深恶痛绝经假手术组雌性大鼠高３０％（Ｐ〈０．０５     

应激刺激对大鼠下丘脑血管升压素mRNA水平的影响

实验在给予慢性应激刺激的Ｓｐｒａｇｕｅ Ｄａｗｌａｙ雄性大鼠中进行,用核酸斑点杂交技术观察大鼠下丘脑组织中血管升压素（ＡＶＰ）ｍＲＮＡ水平变化,用异羟基洋地黄毒甙（ＤＩＧ）标记的２６个碱基长寡聚核苷酸作为检测探针。结果观察到：在给予电击足底结合噪声的应激刺激之后,尾动脉收缩压逐渐升高,到刺激第５天,刺激组与对照组动物之间尾动脉收缩压差别有统计学显著意义;到刺激第９天,刺激组尾动脉收缩压达最高值;以     

异羟基洋地黄毒甙配基核酸探针及其检测系统

<正>原理 异羟基洋地黄毒甙配基(Digoxigenin,以下简称Dig,是从植物洋地黄中提取的固醇类半抗原物质。由连接臂共价结合到嘧啶环的5位上,构成Dig标记的核苷酸类似物Dig-11-dUTP。     

血管紧张素Ⅱ对大鼠下丘脑内血管升压素基因转录的影响

实验在雄性ＳＤ大鼠中进行,用核酸斑点杂交技术观察下丘脑组织中血管升压素（ＡＶＰ）基因转录水平变化,用异羟基洋地黄毒甙（ＧＩＧ）标记的２６个碱基长寡聚核苷酸作为检测探针。实验中观察到,用渗透压微泵向大鼠侧脑人连续注射微量血管紧张素Ⅰ（０．２ｎｍｏｌ／ｈ）２ｄ后,可引起动物饮水量显著增加,下丘脑组织中ＡＶＰ基因转录水平高,但无统计学显著意义。将实验动物日饮水量限制在与对照动物相同的每日饮水量之后,侧脑     

用非放射性原位杂交和免疫金染色在豌豆间期染色质内显示的rDNA的分布

以异羟基洋地黄毒甙标记的ｒＲＮＡ为探针,通过与植物根尖分生组织区振动切片中的ｒＤＮＡ原位杂交,结合免疫金染色及银加强金处理研究了豌豆间期染色质中ｒＤＮＡ的分布。研究结果清楚地显示供试植物间期细胞内有１－５个显著的ｒＲＮＡ探针结合位点,其中显示４个结合位点的细胞占６０．６％,少于和多于４个结合位点的细胞分别上３７．９％和１．１４％。在显示４个结合位点的细胞核内,它们分别按照２：１、３：１和２：１：１     

地高辛素标记的探针快速检测HBV-DNA实验研究

应用核酸分子杂交技术,检测血清中HBV-DNA已成为诊断乙型肝炎病毒感染和判断其复制状态的重要手段。用同位素(~(32)P)标记核酸探针,进行分子杂交,虽然灵敏度高,但是由于具有半衰期短、探针不稳定、价格昂贵、对人体有害等因素,使之推广应用受到限制。目前国内外已有地高辛素(Dig)标记HBV-DNA探针进行斑点杂交实验,敏感性接近同位素探针水平。我们参照BM公司试剂盒方法及有关文献,建立Dig标记HBV基因探针方法,采用随     

A Comparison of Digoxigenin and Biotin Labelled DNA and RNA Probes for in Situ Hybridization

A number of in situ hybridization protocols using digoxigenin or biotin labelled probes were assessed for viral nucleic acid detection in formalin fixed, paraffin embedded tissue. Single-step detection protocols for biotin labelled probes produced low sensitivity; however, enzyme based one-step detection protocols for digoxigenin probes produced high sensitivity for both RNA and DNA systems. For both probe types, multistep detection protocols produced equally high sensitivity. Use of an enhanced APAAP procedure for digoxigenin labelled probes acheived maximal sensitivity without use of biotin-streptavidin reactions. The sensitivity of nucleic acid detection obtained with a digoxigenin labelled probe is comparable to that obtained using biotin. Digoxigenin labelled probes for nucleic acid detection are recommended for tissues with endogenous biotin.     

地高辛精标记酪氨酸羟化酶RNA探针的制备研究

为制备用地高辛精（Ｄｉｇｏｘｉｇｅｎｉｎ,Ｄｉｇ）标记的酶氨酸羟化酶（ＴｙｒｏｓｉｎｅＨｙｄｒｏｘｙｌａｓｅ,ＴＨ）ＲＮＡ探针,本研究用分子生物学技术重组质粒ＰＧＥＭＴＨＩ,即分别将携带Ｔ７和Ｓｐ６启动子的ＰＧＥＭ－３ｚｆ质粒和携带ＴＨ基因的ＰＫＳＴＨ质粒用限制性内切酶消化并行分离纯化,得到带Ｔ７和ｓｐ６启动子的ＤＮＡ片段和ＴＨ基因片段;经Ｔ４ＤＮＡ连接酶连接后转入大肠杆菌,得到ｐＧＥＭＴＨ１重组克隆。经小量提取质粒井用酶切分析检测,证实其确有ＴＨ基因且方向正确。将此质粒再经限制性内切酶消化则得到线状ＤＮＡ片段,用Ｔ７ＲＮＡ聚合酶转录合成带有Ｄｉｇ标记的高比活度的单链ＲＮＡ探针;经斑点杂交试验证实该探针具有较高的可靠性。这将为基因治疗帕金森氏病动物模型的疗效检测提供有效手段。     

Alterations in DNA-dependent RNA polymerase I from rat liver accompanying ethionine administration

Multiple injections of ethionine plus adenine resulted in 3- to 4-fold increases in the activity of RNA polymerase I from rat liver nuclei, whereas the activity of RNA polymerase II was relatively unaffected. Methyl-deficient preribosomal RNA was present in the livers of rats after treatment for 2 days. Both incorporation of labelled orotate into rat liver ribosomal RNA and protein synthesis in polysomes gradually increased.     

RNA在离体小鼠肝脏组织中的稳定性

采取肝脏等临床样本时,常因不能及时保存造成核酸降解,从而影响后续实验的进行.本研究旨在通过对室温条件下放置不同时间的小鼠肝脏组织的RNA的完整性进行评价,为肝脏临床样本的采集与保存提供依据.将离体小鼠肝脏组织在室温下放置0～180min后,提取总RNA,采用电泳、RT-PCR和芯片生物分析仪检测RNA的完整性.电泳结果显示,将小鼠肝脏置于室温180min后,RNA尚未发生降解.对β肌动蛋白,GAPDH和Trp53的RT-PCR的分析表明,室温下保存180min的RNA样品均未降解.生物分析仪检测的RNA完整性系数(RIN)都大于7.9,样品可用于后续研究.因此,离体后的小鼠肝脏置于室温下3h以内,RNA仍能保持其完整性.     

Detection of groundnut rosette umbravirus infections with radioactive and non-radioactive probes to its satellite RNA

A cloned cDNA copy of the satellite RNA of groundnut rosette virus (GRV), labelled with either ³²P or digoxigenin, was used as a probe to detect the satellite RNA in infected leaves. The test was successfully applied to N. benthamiana and to groundnuts, infected with isolates of GRV from East and West Africa and with isolates which cause different types of symptom in groundnuts, including one which is almost symptomless. Although the probe did not react with extracts from plants infected with GRV isolates from which the satellite RNA had been artificially eliminated, all naturally occurring GRV isolates contain the satellite RNA. The test therefore provides a reliable indicator of infection by GRV.     

生物素标记HBV RNA探针的制备及应用

本文首次采用ＳＰ６５特殊质粒与人类的乙型肝炎病毒ＤＮＡ重组,制备了Ｂｉｏ－ＨＢＶ ＲＮＡ探针,能特异地与ＨＢＶ ＤＮＡ杂交,将该探针与缺口转移方法标记的Ｂｉｏ－ＨＢＶ ＤＮＡ探针进行了比较,结果显示出Ｂｉｏ－ＨＢＶ ＲＮＡ探针比Ｂｉｏ－ＨＢＶ ＤＮＡ探针的敏感性提高１０倍,并分别应用两种探针同时检测７０例乙肝病人血清中ＨＢＶ ＤＮＡ,阳性率各为３１．４２％、２８．５７％（Ｐ＞０．２５）。对Ｂｉｏ－     

斑点杂交生物素法检测流行性出血热病毒RNA

为寻找一种用于检测流行性出血热病毒的分子杂交方法,以生物素-7-dATP标记流行性出血热病毒(EHFV)R_(22)株M片段的cDNAR_3克隆作探针,与人源性的EHFVH-114、H-435株RNA基因组进行斑点杂交,得到阳性结果,可检出5pg的cDNA或RNA。此探针与疱疹病毒DNA不出现杂交信号。以上结果说明这种标记探针具有EHFV特异性,可以扩大应用范围,结果还表明动物源性和人源性EHFV均具有共同的保守核苷酸序列。     

RNA recognition by a human antibody against brain cytoplasmic 200 RNA

Diverse functional RNAs participate in a wide range of cellular processes. The RNA structure is critical for function, either on its own or as a complex form with proteins and other ligands. Therefore, analysis of the RNA conformation in cells is essential for understanding their functional mechanisms. However, no appropriate methods have been established as yet. Here, we developed an efficient strategy for panning and affinity maturation of anti-RNA human monoclonal antibodies from a naïve antigen binding fragment (Fab) combinatorial phage library. Brain cytoplasmic 200 (BC200) RNA, which is also highly expressed in some tumors, was used as an RNA antigen. We identified MabBC200-A3 as the optimal binding antibody. Mutagenesis and SELEX experiments showed that the antibody recognized a domain of BC200 in a structure- and sequence-dependent manner. Various breast cancer cell lines were further examined for BC200 RNA expression using conventional hybridization and immunoanalysis with MabBC200-A3 to see whether the antibody specifically recognizes BC200 RNA among the total purified RNAs. The amounts of antibody-recognizable BC200 RNA were consistent with hybridization signals among the cell lines. Furthermore, the antibody was able to discriminate BC200 RNA from other RNAs, supporting the utility of this antibody as a specific RNA structure-recognizing probe. Intriguingly, however, when permeabilized cells were subjected to immunoanalysis instead of purified total RNA, the amount of antibody-recognizable RNA was not correlated with the cellular level of BC200 RNA, indicating that BC200 RNA exists as two distinct forms (antibody-recognizable and nonrecognizable) in breast cancer cells and that their distribution depends on the cell type. Our results clearly demonstrate that anti-RNA antibodies provide an effective novel tool for detecting and analyzing RNA conformation.