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Peer-reviewed veterinary case report

How to diagnose feline herpesvirus skin infection in cats

By Mazzei, Maurizio et al.·Published in Veterinary dermatology·2019·Department of Veterinary Sciences, Italy·View original on PubMed

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Original publication title: Quantitative real time polymerase chain reaction (qRT-PCR) and RNAscope in situ hybridization (RNA-ISH) as effective tools to diagnose feline herpesvirus-1-associated dermatitis.

Species:
cat

Plain-English summary

A group of cats with facial skin issues was tested for feline herpesvirus type 1 (FHV-1) to determine if it was causing their dermatitis. Researchers used advanced testing methods to analyze tissue samples from these cats and found that FHV-1 was present in some cases of dermatitis, while healthy cats and those with other types of skin issues did not show the virus. This means that these testing methods can help veterinarians diagnose FHV-1-related skin problems more accurately, even when typical signs are not visible.

People also search for: cat skin problems · feline herpesvirus dermatitis treatment · how to diagnose cat skin issues

Abstract

BACKGROUND: Felid herpesvirus type 1 (FHV-1)-associated dermatitis is characterized by facial and nasal involvement; clinical and histopathological manifestations may overlap with other dermatitides. OBJECTIVE: To evaluate the realibility of qRT-PCR-2and RNAscope in situ hybridization (RNA-ISH) methods to diagnose FHV-1-associated dermatitis, in formalin-fixed paraffin-embedded (FFPE) tissues. ANIMALS: Sixteen FFPE samples from cats with facial dermatitis and four controls were studied. METHODS AND MATERIALS: Based on histopathological features, cases were separated into: Group 1, samples with herpetic dermatitis (four); Group 2, samples with nonherpetic facial dermatitis (six); Group 3, samples with facial dermatitis of ambiguous nature (allergic or viral) (six); and Group 4, samples from healthy cats (four). A relative quantification using the 2method was used to estimate the "upregulation" of each FHV-1 target viral gene copies (glycoprotein-B and thymidine-kinase) relative to reference gene. Detection of FHV-1 mRNA was performed using the RNAscope 2.5 detection kit. RESULTS: By 2analysis, upregulation of both FHV-1 genes was observed in all samples from Group 1 and two of six from Group 3. No upregulation was identified in samples from groups 2 and 4. Positive mRNA hybridization signal was observed in all cases from Group 1 and two cases of Group 3. No positivity was observed in samples from groups 2 and 4. CONCLUSIONS AND CLINICAL IMPORTANCE: QRT-PCR 2analysis and RNA-ISH can identify the FHV-1 genome as causative agent of the associated dermatitis, even where inclusion bodies are not detectable. Both techniques are functional in retrospective studies, have greater specificity than conventional PCR, and may be proposed for research and diagnostic purposes.

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Original publication on PubMed: https://pubmed.ncbi.nlm.nih.gov/31486555/