The d gene from the Bacillus subtilis temperate bacteriophage SP,3 was isolated. When introduced into an SP,l-sensitive strain of B. subtilis, the cloned d gene directed the synthesis of a 22-kilodalton protein and conferred on the host immunity to SP,i phage. A frameshift mutation, designated d2, was introduced into the cloned d gene, and it was subsequently crossed back into the SPI8 phage genome. The ml when needed, was used as a plating medium for phage and bacteria.Phage growth and DNA preparation. Phage SPI c2 was prepared from strain CU1147 by the heat induction method essentially as described by Rosenthal et al. (13). Wild-type SP,B phage was prepared either by mitomycin C (0.8 ,ug/ml) induction or, as for SP3 clO (described below), by growing phages lytically by the method of Warner et al. (16) with the following modifications: (i) the adsorption period at 37°C was 15 to 20 min; (ii) the centrifugation step to remove unadsorbed phage was omitted; and (iii) infected cells were diluted 30-to 100-fold into prewarmed (37°C) modified M medium.Purified phage particles were prepared by the method of Fink et al. (3) with several modifications. Polyethylene glycol 6000 was added to 10% (wt/vol) to the phage suspension along with NaCl to 0.5 M to precipitate most of the phage particles. Polyethylene glycol-precipitated phage pellets were suspended in CsCl (1.497 g/ml, in a 10 mM trischloride [pH 7.4]-2 mM MgSO4-10 mM CaC12 buffer) without attempting to remove the trace amount of polyethylene glycol and centrifuged to equilibrium with a Beckman Ti 70.1 rotor at 24,500 rpm for 28 h or with a VTi8O rotor at 60,000 rpm for 6.5 h at 18°C. After collection and dialysis of the phage band, phage suspensions were concentrated, and the phage DNA was extracted with TE (10 mM Trischloride [pH 8.0], 1 mM EDTA) buffer-saturated phenol followed by two chloroform extractions and ethanol precipitation.Isolation of clear-plaque SP13 c1O. During the preparation of SPI c+ phage from the SU+3 (SP1) strain, a spontaneous clear-plaque phage (designated SP, c1O) was fortuitously identified. In all the tests performed, SP clO was indistinguishable from SP, cl; they were both used in these studies.Construction of SPO c2 phage DNA library and other molecular cloning methods. Plasmid pLP1201 (11) replicates in both Escherichia coli and B. subtilis, and it was used for the construction of the phage gene library. BamHI and BglII doubly digested SP3 c2 DNA (2.8 ,ug) was ligated to BamHIdigested pLP1201 (1 ,ug) DNA at a final DNA concentration of about 300 xug/ml. E. coli MM294 (9)
