Ultrastructural localization of defined sequences of viral RNA and DNA by in situ hybridization of biotinylated DNA probes on sections of herpes simplex virus type 1 infected cells

Puvion‐Dutilleul, Francine; Puvion, Edmond

doi:10.1002/jemt.1060180403

Cited by 25 publications

(16 citation statements)

References 29 publications

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“…Hybrids were detected with a goat anti-biotin antibody conjugated to 10-nm gold particles (BBInternational). Detection of DNA requires NaOH treatment of the thin sections before hybridization (Puvion-Dutilleul and Puvion, 1991; Puvion-Dutilleul and Pierron, 1992). This treatment was omitted in all our experiments.…”

Section: Methodsmentioning

confidence: 99%

Highly Ordered Spatial Organization of the Structural Long Noncoding NEAT1 RNAs within Paraspeckle Nuclear Bodies

Souquère¹,

Beauclair²,

Harper³

et al. 2010

MBoC

209

228

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Section: Methodsmentioning

confidence: 99%

Highly Ordered Spatial Organization of the Structural Long Noncoding NEAT1 RNAs within Paraspeckle Nuclear Bodies

Souquère¹,

Beauclair²,

Harper³

et al. 2010

MBoC

209

228

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“…Fixation with glutaraldehyde concentrations higher than 1% has been counter-indicated for specimens subjected to in situ hybridization for electron microscopy (Le Guellec 1998) because of interference with the localization of double-stranded DNA. However, hybridization with single-stranded DNA is possible, especially after proteolytic (enzymatic) digestion (Puvion & Puvion 1991). Indeed, the Proteinase K step increased intensity of the in situ hybridization reaction, suggesting that excessive DNA to protein cross-links had been removed.…”

Section: Discussionmentioning

confidence: 99%

Detection of hepatopancreatic parvovirus (HPV) of penaeid shrimp by in situ hybridization at the electron microscope level

Pantoja

Lightner²

2001

Dis. Aquat. Org.

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A post-embedding in situ hybridization procedure was developed to detect hepatopancreatic parvovirus (HPV) of penaeid shrimp at the ultrastructural level. The procedure was optimized using sections of resin-embedded hepatopancreas from HPV-infected juvenile Penaeus monodon and postlarval P. chinensis. The hepatopancreata were fixed using various fixatives, dehydrated, and embedded in the hydrophilic resin Unicryl™. A 592 bp HPV-specific DNA probe, labeled with DIG-11-dUTP, was tested both on semi-thin and ultra-thin sections and examined by light and electron microscopy, respectively. Hybridized probe was detected by means of an anti-DIG antibody conjugated to 10 nm gold particles and subsequent silver enhancement. Hybridization signal intensities were similar with all fixatives tested, but ultrastructure was best preserved with either 2 or 6% glutaraldehyde. Post-fixation with 1% osmium tetroxide improved ultrastructure but markedly decreased hybridization signal and induced non-specific deposition of gold and silver. Under optimized conditions, this technique was used to successfully follow the development of HPV from absorption and transport through the cytoplansm to nuclear penetration, replication and release by cytolysis. The probe signal was consistently observed among necrotic cell debris within the lumen of hepatopancreatic tubules, within the microvillous border of tubule epithelial cells, within the cytoplasm, and within diagnostic HPV intranuclear inclusion bodies. The nucleolus and karyoplasm of patently infected cells (i.e., showing HPV intranuclear inclusion bodies) were almost devoid of signal. Electron-lucent structures, known as intranuclear bodies, commonly found within the virogenic stroma, showed only weak labeling. This is the first use of in situ hybridization to detect HPV nucleic acids with the electron microscope. The technique should be useful for studying the pathogenesis of HPV. KEY WORDS: Parvoviridae · HPV · Ultrastructural in situ hybridization · Transmission electron microscopy · Penaeus monodon · Penaeus chinensis Resale or republication not permitted without written consent of the publisherDis Aquat Org 44: [87][88][89][90][91][92][93][94][95][96] 2001 tion methods including histology, in situ hybridization or PCR (Lightner et al. 1993, Pantoja & Lightner 2000.HPV infection in cultured shrimp has been linked to chronic mortalities during the early larval and/or postlarval stages (Lightner et al. 1993, Spann et al. 1997, and it may result in stunted growth during the juvenile stages (Flegel et al. 1992, Limsuwan 1999. The effect of HPV on adult shrimp is unknown but it may compromise their survival if the infection is severe and if the shrimp is in a highly demanding metabolic state (i.e., during gonad maturation) (D.V.L. unpubl).Currently, HPV is considered as a member of the Parvoviridae ; however, its position within the family still remains uncertain. Apparently HPV shares more similarities with the autonomous parvoviruses than with the arthropod-infecting parv...

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“…A recurring problem with the use of biotinylated probes for in situ hybridization at the light-microscope HIST 25/(~-B level is the presence of endogenous biotin leading to false-positive signal. One report has indicated that this can also be a problem at the ultrastructural level unless proteolytic digestion is performed (Puvion-Dutilleul & Puvion, 1991). Digoxigenin is gaining in popularity as an alternative non-isotopic probe label at the light microscope level, being capable of providing high resolution localization of target sequences with minimal background signal .…”

Section: -2214 9 1993 Chapman and Hallmentioning

confidence: 99%

Intracellular localization of parvovirus B19 nucleic acid at the ultrastructural level by in situ hybridization with digoxigenin-labelled probes

et al. 1993

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Conditions suitable for immunogold detection of digoxigenin-labelled DNA probes hybridized to parvovirus B19-infected erythroid cells embedded in Lowicryl K4M and LR White acrylic resins were established at the electron microscope level. The protocol was initially optimized using a positive control probe for whole human DNA which produced signal over the heterochromatin of all nucleated cells. In cultures harvested 2 days postinfection, B19 nucleic acid was detected mainly within the centrinuclear region of erythroid cells exhibiting characteristic margination of the chromatin. The B19 hybridization signal was largely unaffected by denaturation and was resistant to RNase digestion but sensitive to DNase digestion, indicating that it was mainly single-stranded B19 DNA. Relatively few gold particles were found over crystalline arrays of viral capsids, consistent with the observation that they are composed of mainly 'empty' capsids. B19 nucleic acid was detected in apparent transit from nucleus to cytoplasm through pores in the nuclear membrane. While the sensitivity of this system is limited by the fact that hybridization occurs only at the surface of the section, it is a rapid and specific means of localizing viral nucleic acids with a high degree of resolution.

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Ultrastructural localization of defined sequences of viral RNA and DNA by in situ hybridization of biotinylated DNA probes on sections of herpes simplex virus type 1 infected cells

Cited by 25 publications

References 29 publications

Highly Ordered Spatial Organization of the Structural Long Noncoding NEAT1 RNAs within Paraspeckle Nuclear Bodies

Highly Ordered Spatial Organization of the Structural Long Noncoding NEAT1 RNAs within Paraspeckle Nuclear Bodies

Detection of hepatopancreatic parvovirus (HPV) of penaeid shrimp by in situ hybridization at the electron microscope level

Intracellular localization of parvovirus B19 nucleic acid at the ultrastructural level by in situ hybridization with digoxigenin-labelled probes

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