Abstract

�� In early 2006, a lumpy skin disease (LSD) outbreak has invaded cattle in different localities of Egypt, exerting severe economic losses to livestock industry. Representative specimens (skin biopsies) were collected form nodular skin lesions of infected foreign (imported from Ethiopia, at Ismailia private quarantine) and local cattle (at F ayoum, Menofia and Sharquia governorates). A polymerase chain reaction (PCR) assay was used, as a basic step, for rapid diagnosis of the causative agent in clinical specimens to control sp read of infection in the rest of Egypt. The PCR assay, utilizing a LSDV P32 based primer set, could identify LSDV in all outbreak clinical specimens. The specific PCR amplification products (amplicons) were purified and subjected to direct nucleotide sequencing. Blast search, multipl e alignments and phylogenetic analyses of the nucleotide sequence data revealed that outbreak LSD V is closely related to other capripoxviruses of LSD, sheep pox and goat pox. Selection and processi ng of clinical specimens, methods of DNA isolation, and PCR assay applied in this endeavor, presented a reliable laboratory diagnostic tool for LSDV.