Staphylococcus aureus RN4220, a cloning intermediate, is sometimes used in virulence, resistance, and metabolic studies. Using whole-genome sequencing, we showed that RN4220 differs from NCTC8325 and contains a number of genetic polymorphisms that affect both virulence and general fitness, implying a need for caution in using this strain for such studies.Staphylococcus aureus is a versatile pathogen that is responsible for the majority of nosocomial and community-acquired infections. One of the biggest challenges in treating staphylococcal infections is that many S. aureus strains have developed resistance against various antibiotics. In contrast to clinical isolates, RN4220 is a commonly used laboratory strain that is characterized by a mutation in the sau1 hsdR gene, making it restriction deficient and hence an ideal intermediate cloning host. RN4220 was originally derived from NCTC8325-4 using UV and chemical mutagenesis (10). NCTC8325-4, in turn, was derived from an early clinical isolate, NCTC8325 (also known as PS47 or RN1), cured of three prophages (16). Indeed, RN4220 is not a suitable candidate for the study of antibiotic resistance, because newer methicillin-resistant S. aureus (MRSA) lineages have evolved [e.g., ST239 (hospital), ST80, and ST59 (community)], presumably due to recombination events between lineages. RN4220 is also known to harbor a small deletion in rsbU, a gene within the stress-induced sigB operon, which renders it deficient in B expression. Additionally, RN4220 shows a ⌬agr mutant phenotype and does not produce ␣-hemolysin despite producing small amounts of RNAIII in late log phase (24). Recent studies revealed that a deletion of cvfB (encoding conserved virulence factor B) in RN4220 resulted in diminished agr expression, with a reduction in hla expression, protease production, and virulence, in a silkworm model of systemic infection (14), but the loss of hemolytic activity in the cvfB mutant of RN4220 was found to be due to a defective agr locus and not attributable to the cvfB mutation (14). In another study, SrrAB, a two-component regulatory system, was found to repress the transcription of RNAIII of the agr locus in RN4220 (20,27). However, the interpretation of virulence and of the associated regulatory data in these studies with RN4220 is suspect due to an inherent agr defect in this strain (24). Finally, O'Neill showed by comparative sequencing that NCTC8325-4, which was thought to be identical to its parent NCTC8325 except for the deletion of three prophages, possesses previously undescribed polymorphisms that may influence the virulence and pathogenicity of NCTC8325-4 (18). As a result of these issues, it is extremely important to delineate an accurate picture of the mutations in RN4220, given the polymorphisms in this strain which can have an impact upon virulence and resistance phenotype.Using Illumina Solexa-based whole-genome sequencing (paired end) (P. Mayer, L. Farinelli, and E. Kawashima, U.S. patent application WO98/44151), we obtained the whole-genome sequence of st...
