生长抑素mRNA与神经肽Y，催产素在大鼠前脑内的分布及其共存现象──地高辛标记c－RNA探针原位杂交与免疫组化联合法

本实验应用地高辛标记ｃＲＮＡ探针原位杂交组化和免疫组化联合法在同一切片上先后显示了生长抑素ｍＲＮＡ神经元和催产素神经元,生长抑素ｍＲＮＡ神经元和神经肽Ｙ神经元。结果表明生长抑素ｍＲＮＡ及神经肽Ｙ广泛地共存于大鼠的大脑新皮质,尾壳核,以及海马等处的神经元中。所有位于大脑新皮质,尾壳核处的神经肽Ｙ神经元均含有生长抑素ｍＲＮＡ,部分位于海马的神经肽Ｙ神经元含有生长抑素ｍＲＮＡ,而所有位于下丘脑弓状核,室周核的神经肽Ｙ神经元均不含有生长抑素ｍＲＮＡ;生长抑素ｍＲＮＡ与催产素虽然共同分布于下丘脑许多核区,但未见共存于同一神经元。本文对地高辛标记ｃＲＮＡ探针原位杂交组化以及它与免疫组化联合法的技术问题进行了讨论。     

大鼠脊髓内生长抑素mRNA原位杂交的研究

采用地高辛标记生长抑素反意ＲＮＡ探针经原位杂交和显色后,光学显微镜下观察生长抑素ｍＲＮＡ在大鼠脊髓内的定位。结果显示：脊髓内含有大量呈紫蓝色的生长抑素ｍＲＮＡ阳性神经细胞,岍性磷酸酶反应产生     

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。     

地高辛标记寡核苷酸探针检测大鼠胰岛素mRNA

本实验采用地高辛标记前胰岛素寡核苷酸探针原位杂交组织化学技术,研究了Ｗｉｓｔａｒ大鼠胰腺组织胰岛素基因的表达。实验用Ｗｉｓｔａｒ大鼠５只,胰腺经４％多聚甲醛灌注固定,并在同一固定液中后固定２４ｈ,常规石蜡包埋切片。结果表明,经前胰岛素寡核苷酸探针杂交的胰腺切片中,胰岛Ｂ细胞呈蓝色。杂交反应物位于Ｂ细胞的细胞质和部分核仁中,胞核无色。胰岛其它细胞及胰腺外分泌部腺泡细胞无杂交反应物。对照切片中均无阳性信号出现。结果表明地高辛标记寡核苷酸探针不仅具备非同位素标记探针的优点而且能精确检测特异性ｍＲＮＡ的表达。本研究方法操作便利,可靠精确,重复性好。     

簇毛麦低拷贝cDNA序列的克隆和鉴定

从簇毛麦叶片中提取总ＲＮＡ,进一步分离ｍＲＮＡ。以ｍＲＮＡ为模板反转录合成ｃＤＮＡ,两端经Ｔ４ＤＮＡ多聚酶修平后加ＥｃｏＲ１接头分子,连接于质粒ｐＧＥＭ－７Ｚｆ（＋）的ＥｃｏＲ１克隆位点,转化大肠杆菌ＪＭ１０３菌株建立了ｃＤＮＡ文库。用ＰＣＲ扩增重组质粒的ｃＤＮＡ插入序列,用＾３２Ｐ标记后分别与ＨｉｎｄⅢ或ＸｂａⅠ酶切的小麦－黑麦附加系ＤＮＡ进行Ｓｏｕｔｈｅｒｎ杂交。根据其杂交结果,目前已鉴定出４     

胎脑黑质脑内移植矫正PD鼠纹状体内脑啡肽mRNA过度表达

用６－ＯＨＤＡ损毁大鼠一侧黑质—纹状体通路可引起ＰＤ模型鼠脑纹状体内多巴胺匿乏．同时,亦可导致脑啡肽ｍＲＮＡ过度表达。我们用地高辛标记的ｃＲＮＡ探针对纹状体内脑啡肽ｍＲＮＡ含量进行了斑点杂交定量研究,发现损伤侧脑啡肽ｍＲＮＡ含量较健侧增高８０％,胎中脑移植到失神经支配的纹状体内,脑啡肽ｍＲＮＡ过度表达得以矫正至正常水平,说明胎多巴胺能神经元脑内移植能够调节脑啡肽基因表达,提供了移植物能与宿主发生神经整合、建立突触联系的间接证据。     

原位杂交检测大鼠前庭代偿中GAP-43 mRNA水平

用ＤＩＧ标记的ＧＡＰ－４３ｃＤＮＡ为探针,以大鼠海马切片作阳性对照,使用原位杂交方法检测了大鼠迷路损毁５,１２,２０和３０ｄ后前庭核区ＧＡＰ－４３ｍＲＮＡ水平的变化,结果表明,迷路损毁后前庭核区ｍＲＮＡ水平升高,原位杂交的应用,为前庭代偿中轴突发芽,突触重组的神经可塑性研究打下了方法学基础。     

鳄梨冷藏过程中体外转译和基因表达的研究

鳄梨果实经低温贮藏一定时期,从中提取ＲＮＡ,进行体外转译和同源探针杂交分析,以研究冷藏过程中特写基因的表达时期和水平。并用纯化出的冷藏果实的ｍＲＮＡｓ,构建其ｃＮＤＡ文库。对文库作了初步筛选,２４个含ｃＤＮＡ插入片段的菌落能差示地与贮藏前和７℃贮藏的ｍＲＮＡ合成的探针杂交。３个纤维素酶ｃＤＮＡ能很好杂交,２个与鳄梨乙烯形成酶ｃＤＮＡ有同源性。     

秋水仙素对大鼠前脑生长抑素mRNA表达的影响

本实验用地高辛标记生长抑素（ＳＯＭ）反意。ＲＮＡ探针原位杂交组织化学研究了秋水仙素对大鼠前脑ＳＯＭｍＲＮＡ表达的影响。结果表明秋水仙素对前脑各核区ＳＯＭｍＲＮＡ的表达有明显的影响。结果表明秋水仙素对前脑各核区ＳＤＭｍＲＮＡ的表达有明显的核区特异性：大脑新皮质各区,隔核和脚内核中ＳＯＭｍＲＮＡ阳性神经元数目及含量增加;海马复合体和下丘脑室周核和弓状核中ＳＯＭｍＲＮＡ阳性神经元数目及含量下降;嗅脑,尾壳核和丘脑等核区的则无明显变化、秋水仙素对ＳＯＭｍＲＮＡ表达的核区特异性对正确分析秋水仙素条件下获得的神经肽或神经递质的定位资料具有重要的指导意义。     

大白鼠弓状核内生长抑素mRNA分布的原位杂交组化研究

本文用原位杂交组织化学技术对大鼠下丘脑弓状核内生长抑素ｍＲＮＡ（ＳＯＭｍＲＮＡ）的分布进行研究。发现生长抑素ｍＲＮＡ主要分布于弓状核的神经元胞体及近端树突内。含ＳＯＭｍＲＮＡ的神经元可分为浓染大细胞及淡染小细胞两种类型。结果表明弓状核内某些神经元可以合成生长抑素。     

In situ hybridization methods for the detection of somatostatin mRNA in tissue sections using antisense RNA probes

In situ hybridization studies with [32P] and [3H] labelled antisense RNA probes were undertaken to determine optimal methods of tissue fixation, tissue sectioning, and conditions of hybridization, and to compare the relative merits of the two different radioactive labels. The distribution of somatostatin mRNA in neurons of rat brain using a labelled antisense somatostatin RNA probe was employed as a model for these studies. The highest degree of sensitivity for in situ hybridization was obtained using paraformaldehyde fixation and vibratome sectioning. Optimal autoradiographic localization of mRNA was obtained within 7 days using [32P] labelled probes. However, due to the high energy emittance of [32P], precise intracellular localization of hybridization sites was not possible. [3H] labelled RNA probes gave more precise cellular localization but required an average of 18-20 days autoradiographic exposure. The addition of the scintillator, PPO, decreased the exposure time for the localization of [3H] labelled probes to seven days. We also report a method for combined in situ hybridization and immunocytochemistry for the simultaneous localization of somatostatin in mRNA and peptide in individual neurons.     

Somatostatin gene expression in the thymus gland

A complex pattern of interactions appears to exist between the immune and neuroendocrine systems. Recently, vasopressin, oxytocin and vasoactive intestinal peptide have been isolated from the thymus. Using a rat somatostatin antisense RNA probe we have demonstrated expression of the somatostatin gene in the rat thymus. Furthermore, we have shown that the levels of thymic somatostatin mRNA exhibit a bell-shaped response to dexamethasone administration. Lipocortin I and II antisense RNA probes have been used as a positive control for the effects of the dexamethasone. We would suggest that somatostatin acts in the thymus in a paracrine mode to modulate T lymphocyte development.     

Nonisotopic detection of RNA in an enzyme immunoassay using a monoclonal antibody against DNA-RNA hybrids

A sensitive nonisotopic solution hybridization assay for detection of RNA is described and characterized using a pSP65 plasmid model system. The assay procedure is based on a hybridization reaction in solution between a biotinylated DNA probe and a target RNA. The biotin-labeled hybrids are captured on a microtiter plate coated with an antibody to biotin. Bound DNA-RNA hybrids are detected by an immunoreaction with an enzyme-labeled monoclonal antibody specifically directed against DNA-RNA heteropolymers and the hybrids are quantitatively measured with the addition of a fluorogenic substrate. Optimal conditions under which to perform the assay were hybridization time, 1000 min; temperature, 75 degrees C; probe concentration, 0.2 microgram/ml; extent of probe biotinylation, 6.7%; buffer stringency, 2x SSC. A bisulfite-modified DNA probe was compared to nick-translated probes synthesized with reporter groups of different lengths (bio-11-dUTP or bio-19-dUTP). All probes could detect 10 pg/ml of target RNA. The presence of nonhomologous DNA or RNA sequences reduced the sensitivity of RNA detection by one half-log to 32 pg/ml (1.6 pg/assay).     

mRNA Quantification After Fluorescence Activated Cell Sorting Using Locked Nucleic Acid Probes

Recently, we have established an in-tube in situ hybridization method named mRNA quantification after fluorescence activated cell sorting (FACS-mQ), in which a specific RNA in a particular cell type is stained with a florescent dye, allowing the stained cells to be selected by FACS without suffering excessive RNA degradation. Using this method, the biological characteristics of the sorted cells can be determined by analyzing their gene expression profile. In this study, we used locked nucleic acid (LNA) oligonucleotides, which are known to enhance both the sensitivity and specificity of RNA detection, as hybridization probes in FACS-mQ. When we used a LNA probe targeting the human 28S sequence, we were able to efficiently separate human cells from rat cells. Using LNA probes, the hybridization step was shortened to 1 h. After the hybridization step, 84.6% RNA was preserved; thus, we were able to successfully measure gene expression levels in each type of cell after FACS. Providing the LNA probe efficiently hybridizes with the target sequence, FACS-mQ with an LNA probe is a powerful tool for separating particular cells and determining their biological characteristics by analyzing their gene expression profile.     

High-resolution in situ hybridization to whole-mount zebrafish embryos

The in situ hybridization (ISH) technique allows the sites of expression of particular genes to be detected. This protocol describes ISH of digoxigenin-labeled antisense RNA probes to whole-mount zebrafish embryos. In our method, PCR-amplified sequence of a gene of interest is used as a template for the synthesis of an antisense RNA probe, which is labeled with digoxigenin-linked nucleotides. Embryos are fixed and permeabilized before being soaked in the digoxigenin-labeled probe. We use conditions that favor specific hybridization to complementary mRNA sequences in the tissue(s) expressing the corresponding gene. After washing away excess probe, hybrids are detected by immunohistochemistry using an alkaline phosphatase-conjugated antibody against digoxigenin and a chromogenic substrate. The whole procedure takes only 3 days and, because ISH conditions are the same for each probe tested, allows high throughput analysis of zebrafish gene expression during embryogenesis.     

Combined non-radioactive detection of peptide hormones and their mRNAs in stomach somatostatin cells

Non-radioactive in situ hybridization (ISH) and immunocytochemistry (ICC) have been used to detect somatostatin (SS) messenger RNA (mRNA) and peptide in antropyloric mucosa of the stomach in the rats. We have applied a method of non-radioactive in situ hybridization histochemistry using digoxigenin labelled oligonucleotide probes to detect somatostatin gene expression in the stomach. In prehybridization stage we used proteinase K (PK) in various concentrations (from 1 to 10 micrograms/ml) and periods (from 10 min to 1 h) but we maintained high background. However it was possible to detect the somatostatin mRNAs in the stomach mucosa making use of either background preventing solutions during the prehybridization, or of levamisole (20 microliters/mg) added into the hybridization buffer or of pepsin. Somatostatin mRNA and peptide signals were scattered all through the mucosa especially localized particularly at the base of the pyloric glands. SS peptide shown by ICC and SS mRNA shown by ISH were observed in different cells.