M double-stranded RNA (MdsRNA) plasmid mutants were obtained by mutagenesis and screening of a diploid killer culture partially heat cured of the plasmid, so that a high proportion of the cells could be expected to have only one M plasmid. Mutants with neutral (nonkiller [K-], immune [R+]) or suicide (killer [K+], sensitive [R-]) phenotypes were examined. All mutants became K-Rsensitives on heat curing of the MdsRNA plasmid, and showed cytoplasmic inheritance by random spore analysis. In some cases, M plasmid mutations were indicated by altered mobility of the MdsRNA by agarose gel electrophoresis or by altered size of in vitro translation products from denatured dsRNA. Neutral mutants were of two types: nonsecretors of the toxin protein or secretors of an inactive toxin. Of three neutral nonsecretors examined, one (NLP-1), probably a nonsense mutation, made a smaller protoxin precursor in vitro and in vivo, and two made full-size protoxin molecules. The in vivo protoxin of 43,000 molecular weight was unstable in the wild type and kinetically showed a precursor-product relationship to the processed, secreted 11,000-molecular-weight toxin. In one nonsecretor (N1), the protoxin appeared more stable in a pulse-chase experiment, and could be altered in a recognition site required for protein processing.Killer strains of the yeast Saccharomyces cerevisiae contain M double-stranded RNA (MdsRNA) plasmids encapsidated in a virus-like particle. This MdsRNA codes for a protein toxin and an immunity component. The toxin is secreted and kills sensitive yeast cells devoid of the plasmid (see references 5, 7, and 28 for recent reviews). The toxin appears to be membrane acting (9); it interacts initially with a cell wall receptor (8) and then, in an energy-dependent reaction, causes membrane damage (23). In vitro, in a phospholipid bilayer system, the toxin inserts into the bilayer and forms a pore (B. Kagan, personal communication), and, as in the case of the membrane-acting colicin K (21), this is likely to be the mechanism of action in vivo.The killer toxin system is a useful model for secretion and for events in the interaction of a protein with the cell surface. The existence of mutants in the MdsRNA plasmid that affect toxin or immunity function permits us to make a genetic approach to these problems and to extend work done with chromosomal mutants (1). Although MdsRNA mutations have been described previously (24-26), none but the suppressive sensitive deletions (10) have been examined in detail. Here we examine nine mutants, six defective in toxin activity or secretion and three partially defective in the immunity component.
MATERIALS AND METHODSYeast stains and media. The diploid killer strain T158C/S14a (8) was used as the wild type for the production of mutants and as the killer strain in phenotype tests. Sensitive strains used were S6, K19.10, and A8207NK. Neutral mutants Ni and N2 were also used (24).Growth medium was the minimal medium of Halvorson (11) plus 0.5% yeast extract, 0.5% peptone, and 2% dextrose [YEPD ...
