NCp7 activates HIV-1(Lai) RNA dimerization by converting a transient loop-loop complex into a stable dimer

Nucleocapsid protein 7 (NCp7), the human immunodeficiency virus type 1 (HTV-1) nucleocapsid protein, was shown to strongly potentiate the dimerization of the retroviral genomic RNA. This process involves the inter action of two retroviral RNA monomer subunits near their 5'-ends. A region located upstream from the splice donor site was recently identified as being responsible for the formation of dimeric HIV-1 RNA. This region appeared to be confined within a stem-loop structure, with an autocomplementary sequence in the loop. In an in vitro study of spontaneous dimer formation, we reported that the 77-402 RNA transcript forms two distinct dimers differing in their thermostability: D37 and D55. We identified D37 as a ''kissing'' complex structure, formed via a loop-loop interaction between the two monomers, and D55 as a double stranded structure involving all nucleotides of the stem loop via canonical base pairing. In this report, we have characterized the role of NCp7 in the HIV-1(Lai) RNA dimerization process by using in vitro dimerization assays with RNA transcripts of different lengths and dimer thermal dissociation. Our results show that the nucleocapsid protein NCp7 activates RNA dimerization very likely through interaction with the kissing complex and converts it into a stable dimer. Furthermore, this NCp7-prometed conversion only occurs if the 240-280 stem loop structure is present in HIV-1(Lai) RNA molecules and contains the autocomplementary G(257)CGCGC(262) sequence. This study suggests that, under physiological conditions, an NCp7-mediated RNA conformational change is involved in the maturation of the HIV-1 RNA dimer.