Each time bacteria were scraped off two different
stabs, resuspended in saline, serially diluted and plated on LB agar. Bacteria from a third stab were streaked directly onto an LB plate for a qualitative analysis of the rpoS status. The colonies were then stained with iodine. Figure 2 shows Barasertib clinical trial the evolution of rpoS segregation in the stabs. At day 1, all tested bacteria were rpoS +, but by day 7 onwards, the presence of many low-RpoS colonies became apparent both in the quantitative (CFU count) and qualitative (streaks) plates. The exact proportion of these mutants varied from week to week, but was never lower than 40%. A common and inexpensive alternative to https://www.selleckchem.com/products/ITF2357(Givinostat).html LB-stabs is a bacterial suspension in filter disks in the presence of glycerol. To test this transporting method, a culture of MC4100TF was resuspended in 15% glycerol (v/v) and 0.1 ml of the suspension was applied onto Caspase inhibitor a filter disk, which was placed in
a small plastic bag and sealed. Glycerol filter disks were prepared along with the stabs reported in Figure 2 and stored at room temperature. Every week a pair of disks was removed from their plastic bags suspended in a small volume of saline and streaked on LB agar. Until day 21 all colonies recovered from the filter disks displayed a high-RpoS phenotype (stained dark brown with iodine). From day 31 onward a significant proportion (approx. 50%) of the bacteria recovered from the filter disks were low-RpoS. Furthermore, there was an increasing reduction in the number of colonies recovered every week, possibly due to prolonged starvation and dehydration of the filter disks (despite the sealing of the plastic bags). It is clear, though, that the glycerol filter disks preserved the genetic integrity of the bacteria for a longer period of time than the LB-stabs. Therefore, the use of glycerol filter disks for bacterial shipment is preferable. The data presented here indicate that the use of LB-stabs for the exchange of bacteria between
laboratories is undermined by genetic instability. Alternative storage and shipment forms, such as freeze-drying, glycerol filter disks or dry ice must be considered. Some of them are costly (shipment of glycerol stocks in dry ice) or dependent on specific equipments (lyophiliser) and none is free of drawbacks. As a matter of fact, induction of mutations during the freeze-drying process has been C1GALT1 reported [26, 27]. Glycerol filter disks provide an inexpensive and easy alternative for bacterial shipping. Since the filters lack essential nutrients we expect very little or no bacterial growth and hence a significant reduction in mutant segregation. Ever since the pioneer work of the Kolter group , several papers have reported the occurrence of rpoS mutations that confer selective advantage in stationary phase (the GASP phenotype) [8, 9, 29]. Accordingly, sequence variation of rpoS in E. coli natural isolates is extensively well documented [3, 3, 16, 30–32].