The development of SPPI has been studied in several B. subtilis mutants conditionally defective in initiation of DNA replication. Initiation of SPPI replication is independent of the host DnaA (replisome organizer), DnaI3, DnaC and DnaI products, but requires the DnaG (DNA primase) and the DNA gyrase. Furthermore, SPPI replication is independent of the DnaK (heat shock) protein. The phage-encoded products required for initiation of SPPI replication have been genetically characterized. Analysis of the nucleotide sequence (3292 kilobases) of the region where SPPI initiation replication mutants map, revealed five open reading frames ( orf). We have assigned genes 38, 39 and 40 to three of these orfs, which have the successive order gene 38-gene 39-orf39,1-gene 40-orf41. The direction of transcription of the reading frames, the lengths of the mRNAs as well as the transcription start point, upstream of gene .38 (PE2), were identified. Proteins of 29·9, 14·6 and 46·6 kDa were anticipated from translation of gene 38, gene 39 and gene 40, respectively. The purified G 38P and G 39P have estimated molecular masses of 31 and 15 kDa. G 38P and G 39P do not share significant identity with primary protein sequences currently available in protein databases, whereas G 40P shares substantial homology with a family of DNA primase-associated DNA helicases. G 38P binds specifically to two discrete SPPI DNA restriction fragments (E coRI-4 and , EcoRI-3). The G 38P binding site on EcoRI-4 was localized on a 393 by DNA segment, which lies within the coding sequence of gene 38. The putative binding site on EcoRI-3 was inferred by DNA sequence homology, it maps in a non-coding segment. G 39P, which does not bind to DNA, is able to form a complex: with G 38P. The organization of the SPPI genes in the gene 38 to gene 40 interval resembles that one found in the replication origin regions of different Escherichia coli double-stranded DNA phages (λ, φ80 and P22). We propose that the conserved gene organization is representative of the replication origin region of a primordial phage.