Mus cervicolor murine leukemia virus isolate M813 belongs to a unique receptor interference group.
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Mus cervicolor murine leukemia virus isolate M813 belongs to a unique receptor interference group. / Prassolov, V; Hein, Sybill; Ziegler, M; Ivanov, D; Münk, C; Löhler, J; Stocking, C.
in: J VIROL, Jahrgang 75, Nr. 10, 10, 2001, S. 4490-4498.Publikationen: SCORING: Beitrag in Fachzeitschrift/Zeitung › SCORING: Zeitschriftenaufsatz › Forschung › Begutachtung
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T1 - Mus cervicolor murine leukemia virus isolate M813 belongs to a unique receptor interference group.
AU - Prassolov, V
AU - Hein, Sybill
AU - Ziegler, M
AU - Ivanov, D
AU - Münk, C
AU - Löhler, J
AU - Stocking, C
PY - 2001
Y1 - 2001
N2 - Murine leukemia virus (MuLV) M813 was originally isolated from the Southeast Asian rodent Mus cervicolor. As with the ecotropic MuLVs derived from Mus musculus, its host range is limited to rodent cells. Earlier studies have mapped its receptor to chromosome 2, but it has not been established whether M813 shares a common receptor with any other MuLVs. In this study, we have performed interference assays with M813 and viruses from four interference groups of MuLV. The infection efficiency of M813 was not compromised in cells expressing any one of the other MuLVs, demonstrating that M813 must use a distinct receptor for cell entry. The entire M813 env coding region was molecularly cloned. Sequence analysis revealed high similarity with other MuLVs but with a unique receptor-binding domain. Substitution of M813 env sequences in Moloney MuLV resulted in a replication-competent virus with a host range and interference profile similar to those of the biological clone M813. M813 thus defines a novel receptor interference group of type C MuLVs.
AB - Murine leukemia virus (MuLV) M813 was originally isolated from the Southeast Asian rodent Mus cervicolor. As with the ecotropic MuLVs derived from Mus musculus, its host range is limited to rodent cells. Earlier studies have mapped its receptor to chromosome 2, but it has not been established whether M813 shares a common receptor with any other MuLVs. In this study, we have performed interference assays with M813 and viruses from four interference groups of MuLV. The infection efficiency of M813 was not compromised in cells expressing any one of the other MuLVs, demonstrating that M813 must use a distinct receptor for cell entry. The entire M813 env coding region was molecularly cloned. Sequence analysis revealed high similarity with other MuLVs but with a unique receptor-binding domain. Substitution of M813 env sequences in Moloney MuLV resulted in a replication-competent virus with a host range and interference profile similar to those of the biological clone M813. M813 thus defines a novel receptor interference group of type C MuLVs.
M3 - SCORING: Zeitschriftenaufsatz
VL - 75
SP - 4490
EP - 4498
JO - J VIROL
JF - J VIROL
SN - 0022-538X
IS - 10
M1 - 10
ER -