P. syringae and E. coli

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CHAPTER 6 A comparison of the recd mutant phenotypes of P. syringae and E. coli 6.1 INTRODUCTION The RecBCD complex is essential for recombination mediated repair of double strand breaks (DSBs) of DNA in E. eou (Smith, 1988). It was observed that mutations in reeb and reec genes make E. eou sensitive to DNA damaging agents, like UV, ionizing radiation, and mitomycin C, due to the inability of the mutant strains to repair DSBs. These mutants have low cell viability even when grown at 37 C, presumably also due to the inability to repair DSBs that occur during normal growth. The RecD, the third component of the RecBCD complex, was however dispensable for the repair of DSBs in E. coli, as revealed by the normal level of resistance of reed mutant cells to DNA damaging agents. The reed mutants of E. coli, unlike reeb and reec mutants, exhibit normal viability at 37 C, suggesting that reed probably does not have any important role in the repair process. However, the recd mutants of E. coli have some other interesting properties. The properties include (i) increased plasmid instability (Biek and Cohen, 1986), and formation of linear plasmid DNA (Cohen and Clark, 1986), (ii) changes in plasmid copy number (Seelke et al., 1987), and (iii) increase in adaptive mutation frequency (Foster and Rosche, 1999). The plasmid instability, increase of copy number and formation of linear plasmids in reed mutants was restricted to only certain class plasmids, and is not a general feature. The reed mutants of E. coli were found to be sensitive to DNA damaging agents in combination with other mutations. For example, reed recj double mutant (Lovett et al., 1988) and the reed ree) sbeb sbecd quadruplet mutant were found to be sensitive to UV (Seigneur et al., 1999). Since our study indicated that the reed of P. syringae could complement the reed mutation of E. coli, with respect to A-phage replication and T4 2- phage multiplication, it was interesting to compare other properties 105

between these two organisms. This chapter describes the results of this comparative analysis. 6.2 RESULTS 6.2.1 The P. syringae (S1 is relatively more sensitive to DNA damaging agents To examine the susceptibility of reed mutant of P. syringae to DNA damaging agents, the sensitivity to UV and mitomycin was tested for CS1 and its isogenic parent R5 (Fig 6.1). Sensitivity to UV and mitomycin C was determined as described in Materials and Methods (Chapter 2). The results indicated that the reed mutant of P. syringae is moderately sensitive to both UV and mitomycin C. For example, in presence of 2 I1g/ml mitomycin C the percentage survival of R5 and CS1 strains were 72% and 20%, respectively. 6.2.2 Plasmid instability of (S1 The reed mutations in E. coli are known to affect the copy number of plasmid (Biek and Cohen, 1986). To examine whether this holds true for the psychrotrophic P. syringae, the stability of the plasmids were determined in P. syringae reed mutants. The stability of two broad host range plasmids pufr034 (IncW replicon) and pgl10 (IncP replicon) were tested. The IncW plasmid pufr034 that was found to have a low stability in the R5 strain, exhibited further instability in the reed disrupted mutant CS1. For example, only about 10 and 3.5% of the R5 and CS1 cells, respectively, retained the pufr034 (Kmr) following their growth on nonselective medium for 24 hrs (Table 6.1). On the other hand, pgl10 was very stable in both R5, and CS1 (Fig 6.2). To exclude the possibility that the stability of pgl10 in CS1 is due to the presence of 53% intact reed, that might produce a truncated protein, the stability of pgl 10 was tested in LDD22 (retaining only 31% of intact reed) and WT strains. The LDD22 strain did not l~ose the kanamycin resistance marker of pgl 10 even up to 100 hours of growth on nonselective medium (data not shown). 106

A) -~... > i:: = 100 80 60 --- R5 rfl 40 -o-cst ~ Q 20 0 0 10 20 30 Duration ofuv exposure (seconds) B)... 100 80 > i:: --- R5 40 rfl = -0- CSt Q ~ 20 -~ 60 0 0 1 2 3 Mtomynin (Ilg/m1) Fig. 6.1 The reed mutant of P. syringae is modestly sensitive to DNA damaging agents UV (A) and mitomycin C (B). C51, reed mutant of P. syringae; R5, parental strain of C51. The sensitivity was calculated based on the c. f.u. of bacterial cells following their treatment to the agents as described under Materials and Methods (Chapter 2) 107

Table 6.1 The plasmid pufr034 is more unstable in (51 % of KanT colonies Time (hours) R5(PUFR034) CS1(PUFR034) o 24 18.6 10.34 13.4 3.44 100 ~.~~=_ --~~.----~. 80 60 40 --tr- R5 -- CSI 20 o 20 40 60 80 100 Fig. 6.2 Stability of plasmid pgl10 in P. syringae. (51, reed mutant of P. sydngae; R5, parental strain of (51 108

6~2.3 E. eoli reed gene does not complement the cold sensitivity of (51 Having found that the reed gene of P. syringae complements the reed mutation in the A phage plaque size assay, the ability of E. coli reed to complement the cold sensitivity of (S1 mutant was tested. The plasmid pkb65, which contained the E. coli reed on the broad-host-range cloning vector pgl 10 was mobilized into (S 1 by conjugation, and the TcrKmr transconjugants were selected. The pgl 10 without any insert was also mobilized to (S1 for use as an empty vector control. As shown in Figure 6.3 the E. coli reed failed to restore the growth of (S1 at 4 C. To rule out the possibility that the lack of complementation is due to the lack of expression of E. coli RecD in P. syringae, Western blot analysis was performed using a monoclonal antibody against the E. coli RecD (Amundsen et at., 2000). The Western analysis results indicated that the E. coli ReeD protein is produced in P. syringe at both 22 ( and 4 ( (Fig 6.4). This suggested that the inability of E. coli reed to complement the growth of P. syringae at 4 ( is not due to lack of expression of the protein, but may be due to the lack of functional domain of ReeD, which is required for growth of at low temperature. 6.2.4 E. eoli reed mutants are not cold sensitive In order to examine whether E. coli reed mutants are sensitive for growth at low temperature (e.g. 10-15 C), growth profiles of the E. coli reed mutant (AG12135 (M(4100 recd1901::tn10) at 37 ( and 15 ( were compared with that of isogenic parent M(4100 (Fig. 6.5). As shown in the Figure both strains grew at comparable rates at both the temperatures, suggesting that reed mutants of E. coli are not cold sensitive. Studies by Nichols et at. (1998) revealed that the Tn 10 insertion in (AG12135 has occurred immediately after the 1542 th nucleotide of 1824 nucleotides long ORF of reed, leaving 84% of the gene intact. Since the LDD11 strain of P. syringae that had 83% of the intact reed gene was not cold sensitive, the proficiency of E. coli (AG12135 to grow at low temperature could simply be due to the residual 84% intact reed in this strain. Therefore, another E. coli strain with a mutation at the N-terminal end was tested for its growth at low temperature. The growth profiles of the mutant V222, and its isogenic parent V66, at 37 ( and 15 ( were compared. The V222 strain had a ( to T mutation in the 10 th nucleotide of reed gene, thus changing the 4th codon 109

10 1 ---R5(pGLl 0) Q Q \Q ~ o -O-CSl(pGLlO) 0.1 ---.-CSl(pKB65) 0.01 4-----,...-----,.---------, o 20 40 60 Time (hrs) Fig. 6.3 The E. coli recd gene does not complement the cold sensitivity of C51. Growth profiles of R5(pGL10), C51(pGL10) and C51(pKB65) in AB broth at 4 C have been shown. pgl10, cloning vector alone; pkb65, plasmid containing the E. coli recd. l10

~ ~.f-:.t:;< ~: f-.,.t:;< ~. QiV ~ 0 ~ 0 ~ 0 Qj ~...... \0... $ ~ $$' ~ ~ ~ ~ J~ &~ ~ ~ ~ ~ ~ ~ ~.\S ~ ~ {J {J.Q;i.Q;i.Q;i.Q;i 1 2 3 4 5 6 7 8 $ ~ u... ~F';:i.'!." ReeD Fig. 6.4 E. eou RecD is expressed in P. syringae. The whole cell extracts of various strains were separated by 50S-PAGE on a 7.5% gel and was subjected to western blot analysis using anti RecD monoclonal antibody. MG1655reeD: :Tn 10, reed mutant of E. eou; (51, cold sensitive mutant; R5, parental strain of (51; pkb65, plasmid containing the E. coli reed; pgl10, broad host range cloning vector 111

A) 10 1 0.1 -II- MC4100 WT --0- MC4100recD::TnlO 0.01 o 2 4 Time (hrs) B) 10 1 0.1 -II- MC4100 WT --0- MC4100recD::TnlO 0.01 o 10 20 30 40 Time (hrs) Fig. 6.5 E. CoU with C-terminal disruption of RecD is not cold sensitive. Growth profiles of E. eou wild type strain MC4100 and the reed mutant MC4100 reed1901::tn10 in LB broth at 37 C (A) and 15 C (B) have been shown 112

A) 10 co co I,Q ~ 0 1 0.1 -+-V66 -- - V222 0.01 o 2 4 6 Time (hrs) B) 10 co o I,Q ~ o 1 0.1 -+-V66 -- - V222 0.01 o 10 20 30 Time (hrs) Fig. 6.6 E. Coli with N-terminal disruption of RecD is not cold sensitive. Growth profiles of E. coli wild type strain (V66) and the recd mutant (V222) in LB broth at 37 ( (A) and 15 O( (B) are shown. 13

encoding arginine to TM stop codon. It was observed that the V222 strain also was not cold sensitive, but exhibited slightly slower growth compared to parental strain V66, at both 37 and 15 ( (Fig. 6.6). These results confirmed that the recd mutants of E. coli are not cold sensitive. 6.3 DISCUSSION The study reported in this chapter was carried out for comparison of recd functions in psychrotrophic P. syringae and mesophilic E. coli. The results indicated that P. syringae recd mutant (51, is slightly more sensitive to DNA damaging agents UV and mitomycin C. This is in contrast to the phenotype exhibited by the recd mutant of E. coli, which are resistant to UV and mitomycin ( (Smith, 1988). Since the RecB(D pathway of homologous recombination plays important role in the repair of DSBs caused by UV, it is possible that the P. syringae RecD might have a unique role in the repair of DNA. The recd gene of E. coli could not complement the cold sensitivity of (S1 even though the E. coli RecD is expressed in P. syringae as indicated by Western blot analysis. Therefore it is tempting to speculate that the P. syringae RecD is functionally different from its E. coli counterpart. However, possibilities like the inability of the E.coli RecD to form complex with the RecB and Rec( proteins of P. syringae, or its improper folding in (S1 at low temperature have to be excluded before attributing a low temperature specific functional role for P. syringae RecD. The growth of E. coli strains with mutation at N-terminal end (e.g. V222) and (-terminal end (e.g. (AG 12135) at low temperature (15 C) imply that the recd gene is not essential for low temperature growth in the mesophilic E. coli. 114

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