POSTEMBEDDING IN-SITU HYBRIDIZATION FOR LOCALIZATION OF VIRAL NUCLEIC-ACID IN ULTRA-THIN SECTIONS

被引：32

作者：

LIN, NS ^{[1
]}

CHEN, CC ^{[1
]}

HSU, YH ^{[1
]}

机构：

[1] NATL CHUNGHSING UNIV,AGR BIOTECHNOL LABS,TAICHUNG,TAIWAN

来源：

JOURNAL OF HISTOCHEMISTRY & CYTOCHEMISTRY | 1993年 / 41卷 / 10期

关键词：

EM IN-SITU HYBRIDIZATION; POSTEMBEDDING METHOD; LOWICRYL HM20; ARALDITE; 502; OSMICATED SAMPLES; DIGOXIGENIN LABELED RIBOPROBES; IMMUNOGOLD LABELING; BAMBOO MOSAIC VIRUS;

D O I：

10.1177/41.10.8245409

中图分类号：

Q2 [细胞生物学];

学科分类号：

071009 ; 090102 ;

摘要：

We developed an in situ hybridization technique for localization of plant virus RNA in ultra-thin sections of virus-infected, Lowicryl HM20- or osmium-fixed, Araldite-embedded plant leaf tissues. A digoxigenin-labeled in vitro transcript corresponding to 173 nucleotides at the 3' end of bamboo mosaic virus (BaMV) RNA was used as a riboprobe and the hybrids were detected by incubation with sheep anti-digoxigenin antibody followed by gold-labeled rabbit anti-sheep IgG. Pre-treatment of ultra-thin sections with an etching agent was the critical step in enhancing hybridization signals on Lowicryl-embedded thin sections. Etching combined with K-metaperiodate treatment increased the accessibility of nucleic acids to riboprobes in osmicated Araldite-embedded sections. BaMV RNA was specifically detected within chloroplasts, mitochondria, and nuclei of infected cells. BaMV virions and BaMV-specific electron-dense crystalline bodies were also labeled. The labeling intensity on Lowicryl-embedded samples, in general, was much higher. than that on osmicated Araldite-embedded samples. However, our procedure offers the advantage that it permits labeling of viral nucleic acids in tissues already processed for routine EM and should be applicable for in situ labeling of any cellular nucleic acids.

引用

页码：1513 / 1519

页数：7

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