A Slow-Motility Phenotype Caused by Substitutions at Residue Asp31 in the PomA Channel Component of a Sodium-Driven Flagellar Motor

doi:10.1128/JB.182.11.3314-3318.2000

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Journal of Bacteriology, June 2000, p. 3314-3318, Vol. 182, No. 11
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

A Slow-Motility Phenotype Caused by Substitutions at Residue Asp31 in the PomA Channel Component of a Sodium-Driven Flagellar Motor

Seiji Kojima, Tomokazu Shoji, Yukako Asai, Ikuro Kawagishi, and Michio Homma^*

Division of Biological Science, Graduate School of Science, Nagoya University, Chikusa-ku, Nagoya 464-8602, Japan

Received 3 January 2000/Accepted 17 March 2000

	ABSTRACT

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PomA is thought to be a component of the ion channel in the sodium-driven polar-flagellar motor of Vibrio alginolyticus. Wehave found that some cysteine substitutions in the periplasmicregion of PomA result in a slow-motility phenotype, in which swarmingand swimming speeds are reduced even in the presence of high concentrationsof NaCl. Most of the mutants showed a sodium ion dependence similarto that of the wild type but with significantly reduced motilityat all sodium ion concentrations. By contrast, motility of theD31C mutant showed a sharp dependence on NaCl concentration, witha threshold at 38 mM. The motor of the D31C mutant rotates stably,as monitored by laser dark-field microscopy, suggesting that themutant PomA protein is assembled normally into the motor complex.Mutational studies of Asp31 suggest that, although this residueis not essential for motor rotation, a negative charge at thisposition contributes to optimal speed and/or efficiency of themotor.

	TEXT

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Flagella are the filamentous organelles responsible for motility of most bacteria. Flagellar rotation is driven by a reversiblerotary motor embedded in the cytoplasmic membrane at the baseof each flagellar filament. The energy for rotation of the flagellarmotors comes from the electrochemical gradient of specific ionsacross the cytoplasmic membrane (protons in Escherichia coli andSalmonella enterica serovar Typhimurium, or sodium ions in Vibriospp. and alkalophilic Bacillus strains) (4, 11, 12, 17).

The essential component for energy conversion in the motor is thought to be a force-generating unit that functions as an ionchannel and interacts with the coupling ion to produce mechanicalforce. In the proton-driven motor, the channel is composed ofa complex of MotA and MotB (5, 9, 10, 25, 27, 28),membrane proteins with four and one single transmembrane segments,respectively (6, 7, 26, 31). It is believed that thecytoplasmic domain of MotA interacts electrostatically with theC-terminal domain of the rotor protein FliG (19, 32). Fourproteins, PomA, PomB, MotX, and MotY, are essential for rotationof the sodium-driven polar-flagellar motors of the marine bacteriaVibrio alginolyticus (1, 8, 23) and Vibrio parahaemolyticus(13, 20, 21). PomA and PomB are homologs of MotA and MotBand are thus thought to form a sodium channel in the motor. Thefunctions of MotX and MotY are unknown, although MotX may alsobe a sodium channel component of the motor, because overproductionof MotX is lethal in E. coli in proportion to the external sodiumion concentration, and also because this lethality is suppressedby the addition of amiloride, a specific inhibitor of the sodium-drivenmotor (20). Mutations resistant to phenamil, an amiloride analog,were recently identified in PomA and PomB, and these mutationsshowed synergistic effects on motility (13, 15). In addition,PomA could be coprecipitated with PomB by anti-PomB antibody,and PomB could be coprecipitated with PomA by anti-PomA antibody(30). These results support the hypothesis that PomA and PomBform a complex. Recently, it has been shown directly that thecomplex consisting of PomA and PomB catalyzes sodium influx inreconstituted proteoliposomes (24).

Slow-motility mutants caused by mutations in MotA have been isolated in E. coli and Salmonella serovar Typhimurium (5,29). It was reported that in most of the slow-motility mutantsmotor torque was normal at low speeds but reduced at high speeds.These mutants generated approximately equal torques in H₂O andD₂O, but their swimming speeds were significantly reduced in D₂Ocompared with those in H₂O (5). These results suggested thatmotor rotation is kinetically limited in these mutants by a processthat might involve proton transfer. In the case of the sodium-drivenmotor, rates of sodium ion flux are easily altered by changingthe NaCl concentration or by using sodium channel-specific inhibitors.This approach allows a direct assessment of the relationship betweenslow rotation and ion flux through the motor. We have generateda series of cysteine-substituted mutations in the periplasmicresidues of PomA and found that some of these mutants show a slow-motilityphenotype (2). In this study, one of these slow-motility mutants,which could not swim in a low concentration of NaCl, wascharacterized.

The PomA mutation D31C causes slow polar flagellar motility. We first examined the relationship between swimming speed and NaCl concentration in the slow-motility pomA mutants isolatedpreviously. The plasmid pYA301 (pomA⁺ Km^r) (15) containing wild-type or mutant pomA was introduced intothe V. alginolyticus strain NMB188 (Laf PomA Che) (15) and cultured to late logarithmic phase at 30°C in VPGmedium (1% polypeptone, 0.4% K₂HPO₄, 3% NaCl, 0.5% glycerol).Swimming speeds were measured in TMN medium containing 50 mM Tris-HCl(pH 7.5), 5 mM MgCl₂, 5 mM glucose, and various concentrationsof NaCl and KCl to keep the sum of the concentrations of NaCland KCl at 300 mM. Most of the slow-motility mutants obtainedby cysteine substitutions in the periplasmic residues of PomAshowed a dependence on sodium ion concentration similar to thatof the wild-type strain, but with swimming speeds significantlylower than for the wild-type strain (Fig. 1A; PomA I175C is atypical example). Among the slow-motility mutants, only D31C showeda significantly different dependence on sodium ion concentration(Fig. 1A). This mutant did not swim at low concentrations of NaCl(0 to 19 mM). It could swim in medium containing 38 mM NaCl, andits swimming speed increased gradually as the concentration ofNaCl in the medium increased. It swam at about 20 µm/s in 300mM NaCl, a speed about one-fourth that of cells expressing thewild-type PomA and comparable to the speed of the PomA I175C mutant.As shown in Fig. 1B, Asp31 of PomA is thought to be located inthe periplasmic loop region. We found that the swimming speedof the PomA D31C mutant was further reduced by the sulfhydrylmodifying reagents dithionitrobenzoic acid and N-ethylmaleimide,although motility of the wild-type strain, which does not containcysteine in PomA, was not reduced. This result suggests that thisresidue is exposed to the outside (2).

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FIG. 1. Sodium concentration dependence of slow-motility mutants. (A) NMB188 (PomA Che) cells containing wild-type (filled circle) or mutant (I175C [triangle] or D31C [open circle]) pomA cells were harvested in late logarithmic phase and resuspended in TMN medium (pH 7.5) containing various concentrations of NaCl. Motility of the cells was observed at room temperature under a dark-field microscope and recorded on videotape. Swimming speed was determined as described previously (3). The average swimming speed was obtained by measuring more than 20 swimming tracks. (B) The predicted transmembrane regions of PomA. The residue Asp31 is marked by a filled circle and white letter. The topology of PomA was predicted from the hydropathy profile of PomA and the topology of the MotA protein of E. coli (31).

Site-directed mutagenesis of PomA Asp31. Given the presumed location of Asp31 in the periplasmic space (Fig. 1B), the negative charge of this residue might affectrates of ion influx through the motor. We next carried out site-directedmutagenesis to replace Asp31 of PomA with various residues. Mutationswere made in pomA carried in the plasmid pYA301 by the two-stepPCR method described previously (15). Plasmids carrying themutated pomA were transformed to the PomA Che strain NMB188, and swimming speeds were measured at various NaClconcentrations (Fig. 2). We generated 10 new mutants, all of which,except the D31F mutant, exhibited motility at 300 mM NaCl. Themutants were classified into four groups according to their NaClthresholds for motility and their maximal swimming speeds in 300mM NaCl. The type I mutant D31E showed nearly the same sodiumdependence and swimming speed as the wild-type strain. Type IImutants were slightly shifted in their threshold for motility,being motile in 13 to 19 mM NaCl, and they exhibited a reducedmaximal swimming speed relative to the wild-type strain. Mutantscarrying substitutions with neutral side chains (D31N, D31Q, andD31S) fell into this group. The single type III mutant (D31G)showed the same NaCl dependence and maximum speed as D31C. TypeIV mutants had a higher NaCl threshold for motility, requiringmore than 75 mM NaCl for motility and showing reduced maximumswimming speeds relative to D31C. Substitution with small (D31A),large (D31Y), or positively charged residues (D31K and D31R) producedthis profile. These results show that various mutations in Asp31of PomA affect the sodium ion concentration dependence of motility.Charge-reversed mutations (D31K and D31R) greatly reduced motility,but the charge-conserved mutation (D31E) did not affect motilityvery much, suggesting that a negative charge at this positionmight be important for optimal function of the motor.

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FIG. 2. Sodium-dependent motility of the PomA Asp31 mutants. Mutants were classified into four groups based on the Na⁺ concentration threshold for motility. NMB188 cells expressing each mutant PomA were harvested at late logarithmic phase and suspended in TMN medium containing various concentrations of NaCl. Swimming speeds were measured as described in the legend to Fig. 1. WT, wild type.

To investigate whether Asp31 is located near ion-binding sites in the channel complex, we examined the inhibition of motilityof the D31C mutant by the sodium channel-specific inhibitors phenamiland amiloride. Motility of both the D31C mutant and the wild-typestrain was inhibited by 50 µM phenamil or 3 mM amiloride in 100mM NaCl (data not shown). Thus, Asp31 of PomA might not be directlyinvolved in binding sodium ions. We also performed immunoblottingof whole-cell proteins of the mutants, using a polyclonal anti-PomApeptide antibody. All of the mutant PomA proteins were detectedat levels sufficient to support motor function (data notshown).

Analysis of speed fluctuations in the PomA D31C mutant. It has been shown, by adjusting the sodium ion concentration in the medium, that rotation of the polar flagellar motor ofV. alginolyticus is stable as the motor speed is varied over awide range (from about 50 to about 1,000 revolutions per second[rps]) (22). Thus, if sodium flux is reduced in the D31C motorbut other aspects of function are unaffected, the rotation speedof the motor should not fluctuate. However, if the force-generatingunits of the mutant bind unstably to sites in the motor, thiseffect should slow the motility and increase fluctuations in rotationspeed. To test this idea, we measured flagellar rotation in NMB188cells containing wild-type or D31C mutant PomA protein by usinglaser dark-field microscopy (LDM), as described previously (16).In this method, a rapidly rotating flagellum is irradiated bya thin beam of laser light, and its rotation rate is measuredfrom the intensity change of scattered light (18).

NMB188 cells containing wild-type or D31C PomA protein were harvested at late logarithmic phase, washed once with TMN medium,and resuspended in the same medium. The cell suspension was pouredinto the space between the slide and the cover glass on whichthin spacers were placed. After 10 min, cells not stuck to thecover glass were washed by a flow of TMN medium. To allow speedfluctuations to be compared at the same average rotation speed,wild-type cells were studied in 6 mM NaCl and mutant cells werestudied in 300 mM NaCl. Figure 3A shows the intensity of scatteredlight versus time for both the wild type and the mutant. Bothmutant and wild-type flagella rotated steadily at about 200 rps(Fig. 3B). To evaluate speed fluctuations of the motors, we madethe following calculation for multiple samples: (standard deviationof the rotation rate)/(average rotation rate) × 100. This valuewas 10 and 12% for the wild type and the D31C mutant, respectively,suggesting that force-generating units of the mutant D31C motorare stably bound to the motor.

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FIG. 3. Flagellar rotation of wild-type and D31C mutant cells detected by LDM. Rotation of a single polar flagellum of a stuck cell of NMB188 expressing wild-type or D31C PomA protein was measured by using LDM for about 6 s in the presence of 6 mM NaCl (wild type) or 300 mM NaCl (D31C), as described previously (16). (A) Intensity changes of the scattered light from the rotating flagellum. The interval between peaks corresponds to the rotation period. (B) Fluctuations in rotation rate of the wild-type and D31C mutant motors plotted as the reciprocal of the interpeak intervals from the data in panel A. Average rotation rates were 197 ± 20.7 rps (wild type) and 187 ± 16.9 rps (D31C).

Possible role of negative charge of Asp31 for motor rotation. In this study, we characterized slow-motility mutants that might have defects in essential steps of torque generation by theflagellar motor. Two questions are raised by these slow-motilitymutants. First, what slows the rotation of these mutant motors?Second, what causes a threshold for motility? Two factors arelikely to be important: the rate of sodium influx through themotors and the efficiency of energy conversion in the motors.That is, ion flux through the mutant motors might be decreasedand/or the efficiency of energy coupling in the mutant motorsmight be reduced by defects in the channel complex. The simplestmodel for such a defect is that mutation of Asp31 of PomA makesions pass more slowly through the channel (for example, the poresize might become smaller). Mutations might reduce the rate offlow so much that it results in a threshold for motility. Similarly,reduction in the efficiency of energy conversion in the motormight cause thisphenotype.

Based on this study, we cannot conclude which model is more likely to explain the effect on motor rotation imposed by replacementsof Asp31. Asp31 is located in the first periplasmic loop (loop_1-2)of PomA, and it has been suggested that loop_1-2 may be in contactwith other proteins, such as PomB, MotX, or MotY, or that it maybe embedded in the pore region of the channel (2). In eithercase, the negative charge of this residue appears to be important.Introduction of a positive charge (D31K or D31R), and also changesin the size of the side chain (D31A and D31Y), caused large increasesin the threshold NaCl concentration needed for motility. Thesemutations (type IV) probably do not cause unstable binding ofthe force-generating units to the motor, because the motors ofD31C mutant rotated steadily. Thus, the mutant phenotype is probablydue to defects in the channel complex itself and not in its installationinto themotor.

The periplasmic segment of PomA contains two other negative charges, D170 and D171 (in loop_3-4). These negative charges, togetherwith D31, may function to recruit sodium ions into the channelcomplex. An analogous recruitment mechanism for hydrogen ionshas been suggested for bacteriorhodopsin (14). The D170C orD171C single mutant reduced motility; however, both of them didnot have NaCl thresholds for motility as D31C did. Double mutationsof these two residues might affect motility more severely. Accordingto sequence alignment of MotA proteins, these three residues areconserved in some species, but not perfectly. Alignment also showsthat MotA proteins have several charged residues in periplasmicdomains, and in most cases, their net charges are negative. Thismight imply that the negatively charged area in MotA proteinscan function similarly to recruit protons into MotA/MotBchannels.

Recently, our group succeeded in measuring sodium ion flux, in response to a potassium diffusion potential, through purifiedPomAB channel complexes reconstituted in proteoliposomes (24).Such a direct measurement of the current passed through the channelcomplex will be needed to clarify the function of residue Asp31.We hope to determine the cause(s) of the Na⁺ concentration threshold and thus gain insight into the mechanismof torquegeneration.

	ACKNOWLEDGMENTS

We thank David F. Blair and Ken Sato for critically reading themanuscript.

This work was supported in part by grants-in-aid for scientific researches (to I.K. and M.H.) from the Ministry of Education,Science and Culture of Japan and the Japan Society for the Promotionof Science (to S.K. and Y.A.).

	FOOTNOTES

^* Corresponding author. Mailing address: Division of Biological Science, Graduate School of Science, Nagoya University, Chikusa-ku,Nagoya 464-8602, Japan. Phone: 81-52-789-2991. Fax: 81-52-789-3001.E-mail: g44416a{at}nucc.cc.nagoya-u.ac.jp.

Present address: Department of Biology, University of Utah, Salt Lake City, UT84112.

REFERENCES

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Abstract
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2. Asai, Y., T. Shoji, I. Kawagishi, and M. Homma. 2000. Cysteine-scanning mutagenesis of the periplasmic loop regions of PomA, a putative channel component of the sodium-driven flagellar motor in Vibrio alginolyticus. J. Bacteriol. 182:1001-1007[Abstract/Free Full Text].

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11. Hase, C. C., and J. J. Mekalanos. 1999. Effects of changes in membrane sodium flux on virulence gene expression in Vibrio cholerae. Proc. Natl. Acad. Sci. USA 96:3183-3187[Abstract/Free Full Text].

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13. Jaques, S., Y. K. Kim, and L. L. McCarter. 1999. Mutations conferring resistance to phenamil and amiloride, inhibitors of sodium-driven motility of Vibrio parahaemolyticus. Proc. Natl. Acad. Sci. USA 96:5740-5745[Abstract/Free Full Text].

14. Kimura, Y., D. G. Vassylyev, A. Miyazawa, A. Kidera, M. Matsushima, K. Mitsuoka, K. Murata, T. Hirai, and Y. Fujiyoshi. 1997. Surface of bacteriorhodopsin revealed by high-resolution electron crystallography. Nature 389:206-211[CrossRef][Medline].

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1.	Asai, Y., S. Kojima, H. Kato, N. Nishioka, I. Kawagishi, and M. Homma. 1997. Putative channel components for the fast-rotating sodium-driven flagellar motor of a marine bacterium. J. Bacteriol. 179:5104-5110[Abstract/Free Full Text].
2.	Asai, Y., T. Shoji, I. Kawagishi, and M. Homma. 2000. Cysteine-scanning mutagenesis of the periplasmic loop regions of PomA, a putative channel component of the sodium-driven flagellar motor in Vibrio alginolyticus. J. Bacteriol. 182:1001-1007[Abstract/Free Full Text].
3.	Atsumi, T., Y. Maekawa, T. Yamada, I. Kawagishi, Y. Imae, and M. Homma. 1996. Effect of viscosity on swimming by the lateral and polar flagella of Vibrio alginolyticus. J. Bacteriol. 178:5024-5026[Abstract/Free Full Text].
4.	Blair, D. F. 1995. How bacteria sense and swim. Annu. Rev. Microbiol. 49:489-522[CrossRef][Medline].
5.	Blair, D. F., and H. C. Berg. 1990. The MotA protein of E. coli is a proton-conducting component of the flagellar motor. Cell 60:439-449[CrossRef][Medline].
6.	Chun, S. Y., and J. S. Parkinson. 1988. Bacterial motility: membrane topology of the Escherichia coli MotB protein. Science 239:276-278[Abstract/Free Full Text].
7.	Dean, G. E., R. M. Macnab, J. Stader, P. Matsumura, and C. Burks. 1984. Gene sequence and predicted amino acid sequence of the motA protein, a membrane-associated protein required for flagellar rotation in Escherichia coli. J. Bacteriol. 159:991-999[Abstract/Free Full Text].
8.	Furuno, M., N. Nishioka, I. Kawagishi, and M. Homma. 1999. Suppression by the DNA fragment of the motX promoter region on long flagellar mutants of Vibrio alginolyticus. Microbiol. Immunol. 43:39-43[Medline].
9.	Garza, A. G., R. Biran, J. A. Wohlschlegel, and M. D. Manson. 1996. Mutations in motB suppressible by changes in stator or rotor components of the bacterial flagellar motor. J. Mol. Biol. 258:270-285[CrossRef][Medline].
10.	Garza, A. G., P. A. Bronstein, P. A. Valdez, L. W. Harris-Haller, and M. D. Manson. 1996. Extragenic suppression of motA missense mutations of Escherichia coli. J. Bacteriol. 178:6116-6122[Abstract/Free Full Text].
11.	Hase, C. C., and J. J. Mekalanos. 1999. Effects of changes in membrane sodium flux on virulence gene expression in Vibrio cholerae. Proc. Natl. Acad. Sci. USA 96:3183-3187[Abstract/Free Full Text].
12.	Imae, Y., and T. Atsumi. 1989. Na⁺-driven bacterial flagellar motors. J. Bioenerg. Biomembr. 21:705-716[CrossRef][Medline].
13.	Jaques, S., Y. K. Kim, and L. L. McCarter. 1999. Mutations conferring resistance to phenamil and amiloride, inhibitors of sodium-driven motility of Vibrio parahaemolyticus. Proc. Natl. Acad. Sci. USA 96:5740-5745[Abstract/Free Full Text].
14.	Kimura, Y., D. G. Vassylyev, A. Miyazawa, A. Kidera, M. Matsushima, K. Mitsuoka, K. Murata, T. Hirai, and Y. Fujiyoshi. 1997. Surface of bacteriorhodopsin revealed by high-resolution electron crystallography. Nature 389:206-211[CrossRef][Medline].
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