Tropism of subgroup J avian leukosis virus as detected by in situ hybridization

SS Arshad, LM Smith, K Howes, PH Russell… - Avian …, 1999 - Taylor & Francis
SS Arshad, LM Smith, K Howes, PH Russell, K Venugopal, LN Payne
Avian Pathology, 1999Taylor & Francis
The HPRS-103 strain of avian retrovirus is the prototype of subgroup J avian leukosis virus
(ALV-J) and causes myeloid leukosis in meat-type chickens. Using immunohistochemical
detection of the viral groupspecific antigen (Gag) we have previously demonstrated that the
induction of myeloid leukosis by ALV-J is associated with viral tropism for myelomonocytic
cells. In this paper we describe an in situ hybridization (ISH) technique using digoxigenin
(DIG)-labelled probes for detecting RNA transcripts in tissues from chickens infected with …
The HPRS-103 strain of avian retrovirus is the prototype of subgroup J avian leukosis virus (ALV-J) and causes myeloid leukosis in meat-type chickens. Using immunohistochemical detection of the viral groupspecific antigen (Gag) we have previously demonstrated that the induction of myeloid leukosis by ALV-J is associated with viral tropism for myelomonocytic cells. In this paper we describe an in situ hybridization (ISH) technique using digoxigenin (DIG)-labelled probes for detecting RNA transcripts in tissues from chickens infected with avian leukosis viruses (ALV) of subgroups J (HPRS-103 strain) and A (RAV-1 strain). Virus-specific RNA was detected mainly in the heart, kidney, proventriculus and adrenal in locations similar to those of the Gag protein. Viral gene expression could not be detected in the bone marrow or tumour tissues using this test. Higher levels of viral gene expression in the bursa of Fabricius infected with RAV-1, but not with HPRS-103, might help explain the inability of the latter virus to induce lymphoid leukosis.
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