Two Nucleotide Transport Proteins in Chlamydia trachomatis, One for Net Nucleoside Triphosphate Uptake and the Other for Transport of Energy

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Journal of Bacteriology, February 1999, p. 1196-1202, Vol. 181, No. 4
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Two Nucleotide Transport Proteins in Chlamydia trachomatis, One for Net Nucleoside Triphosphate Uptake and the Other for Transport of Energy

J. Tjaden,¹ H. H. Winkler,² C. Schwöppe,¹ M. Van Der Laan,¹ T. Möhlmann,¹ and H. E. Neuhaus¹^,^*

Pflanzenphysiologie, Universität Osnabrück, D-49069 Osnabrück, Germany,¹ and Laboratory of Molecular Biology, Department of Microbiology and Immunology, University of South Alabama College of Medicine, Mobile, Alabama 36688²

Received 15 October 1998/Accepted 29 November 1998

	ABSTRACT

Top Abstract Introduction Materials and methods Results Discussion References

The genome of Chlamydia trachomatis, one of the most prominent human pathogens, contains two structural genes coding for proteins,herein called Npt1_Ct and Npt2_Ct (nucleoside phosphate transporters1 and 2 of C. trachomatis), exhibiting 68 and 61% similarity,respectively, to the ATP/ADP transporter from the intracellularbacterium Rickettsia prowazekii at the deduced amino acid level.Hydropathy analysis and sequence alignments suggested that bothproteins have 12 transmembrane domains. The putative transporterswere expressed as histidine-tagged proteins in Escherichia colito study their biochemical properties. His₁₀-Npt1_Ct catalyzedATP and ADP transport in an exchange mode. The apparent K_mvalues were 48 (ATP) and 39 (ADP) µM. ATP and ADP transport wasspecific since AMP, GTP, CTP, UTP, dATP, dCTP, dGTP, and dTTPdid not inhibit uptake. In contrast, His₁₀-Npt2_Ct transportedall four ribonucleoside triphosphates with apparent K_mvalues of 31 µM (GTP), 302 µM (UTP), 528 µM (CTP), and 1,158 µM(ATP). Ribonucleoside di- and monophosphates and deoxyribonucleotideswere not substrates. The protonophore m-chlorocarbonylcyanidephenylhydrazone abolished uptake of all nucleoside triphosphatesby Npt2_Ct. This observation indicated that His₁₀-Npt2_Ct acts asa nucleosidetriphosphate/H⁺ symporter energized by the proton motive force across the Escherichiacoli cytoplasmic membrane. We conclude that Npt1_Ct provides chlamydiaewith energy whereas Npt2_Ct catalyzes the net uptake of ribonucleosidetriphosphates required for anabolicreactions.

	INTRODUCTION

Top Abstract Introduction Materials and methods Results Discussion References

The bacterial genus Chlamydia comprises four species which live as intracellular parasites in specialized vacuoles withineukaryotic cells (reviewed in reference 22). Chlamydia trachomatisis a human pathogen that infect mucous membranes in the urogenitalepithelium and is the leading cause of sexually transmitted diseases.The chlamydial genome (1,043 kbp) is among the smallest of allknown prokaryotic genomes (21). Such reduction of the genomesize of obligate intracellular bacteria is possible because manyintermediates required for their metabolism need not be synthesizedby the complex pathways characteristic of free-living bacteriabut are transported from the intermediate-rich host cell cytoplasmby unusual transport systems that often have no counterparts infree-living bacteria (16, 32).

Both chlamydiae (8) and Rickettsia prowazekii (30), another obligate intracellular bacterial parasite, are able to exchangetheir intracellular ADP for the host cell's ATP. This is a systemin which the net result is the transport of energy for the benefitof the parasite. The ATP/ADP transporter in R. prowazekii (R.prowazekii translocase [RpTLC]) comprises 497 amino acids andbelongs to the family of solute transporters exhibiting 12 transmembranedomains (3, 29). Recently, two functional homologues to therickettsial ATP/ADP transporter have been identified at the molecularlevel in higher-plant plastids from Arabidopsis thaliana (10,15). The amino acid sequences of the plastidic ATP/ADP transportersexhibit 62 to 66% similarity to the evolutionarily widely distantrickettsial ATP/ADP transporter. The plastidic transporters, likethe rickettsial homologue, catalyze ATP import in exchange toendogenous ADP (18).

It has been demonstrated that C. psittaci exhibits an ATP/ADP exchange similar to that in R. prowazekii (8). As both bacterialspecies are obligate intracellular parasitic bacteria but livein very different environmental niches (rickettsiae in the eukaryoticcytosol, chlamydiae in a modified phagosome), it is of interestto identify the transporter protein mediating ATP and ADP movementacross the chlamydial cell membrane. From information availablefrom the C. trachomatis genome program, it became evident thattwo putative membrane proteins with substantial homology to therickettsial ATP/ADP transporter are encoded in the genome (24).

The demonstration that both rickettsial and plastidic ATP/ADP transporters can functionally be expressed in Escherichia coli(3, 12, 15, 27) suggested that this heterologous expressionsystem could also be used to examine the putative chlamydial transporters.In this approach, we amplified the two structural chlamydial genesvia PCR, cloned and expressed the products in E. coli, and analyzedthe nucleotide transport properties of the chlamydial proteinsacross the E. coli cytoplasmic membrane. In this study we characterizedthe biochemical properties of both transporters, with specialattention to whether both structural genes, C. trachomatis npt1(nucleoside phosphate transporter 1) (npt1_Ct) and C. trachomatisnpt2 (npt2_Ct), encode ATP/ADP transport proteins. Answers to thesequestions are crucial for understanding the physiology of oneof the major humanpathogens.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and methods Results Discussion References

Cloning of Npt1_Ct and Npt2_Ct. Genomic C. trachomatis DNA (from serovar L2) was kindly provided by Grant McClarty (University of Manitoba, Winnipeg, Manitoba,Canada). DNA manipulations were performed essentially as describedpreviously (20). The structural genes encoding Npt1_Ct and Npt2_Ctwere amplified from the genomic DNA of C. trachomatis by PCR usingPfu DNA polymerase (Stratagene, Heidelberg, Germany), which hasproofreading activity. The sense primers used, JT100 (5'-catatgactcaaaccgcggaaaaacc-3')and JT200 (5'-tagattaggaaggagcatatgtcttccgagg-3'), were constructedon the basis of data from the C. trachomatis genome program withNdeI restriction sites at the start codons of npt1_Ct and npt2_Ct,respectively. The antisense primers, JT101 (5'-ttaagaaacaccttctatagcaggagcgg-3')and JT201 (5'-ctataaagttgttacaggttcttctcgagac-3'), contained thestop codons of npt1_Ct and npt2_Ct, respectively. The PCR productsobtained for npt1_Ct and npt2_Ct were gel purified and cloned intothe EcoRV site of plasmid pBSK (Stratagene); the resulting plasmidswere named pJT144 and pJT157, respectively. Both DNAs were sequencedon both strands by chain termination reaction (MWG-Biotech, Ebersberg,Germany). To construct E. coli plasmids expressing an N-terminalhistidine tag (pJT167 [encoding His₁₀-Npt1_Ct] and pJT168 [encodingHis₁₀-Npt2_Ct]), the NdeI/BamHI DNA inserts of plasmids pJT144and pJT157 were introduced in frame into the NdeI/BamHI sitesof the isopropyl- $beta$ -D-thiogalactopyranoside (IPTG)-inducible T7RNA polymerase bacterial expression vector pET16b (Novagen, Heidelberg,Germany). Transformation of E. coli was carried out accordingto standardprotocols.

Heterologous expression of ntp1_Ct and ntp2_Ct in E. coli. E. coli C43 cells transformed with plasmid pJT167 or pJT168 were grown in YT-ampicillin medium to an optical density (OD;A₆₀₀) of 0.6. Induction of T7 RNA polymerase was initiated byaddition of IPTG (final concentration, 1 mM). Cells were grownto an OD of 1.3 and collected by centrifugation for 8 min at 5,000× g (4°C). The sediments were resuspended to an OD of 1.0 in potassiumphosphate (50 mM, pH 7.5) (12) and stored on ice until use within1h.

Uptake of radioactively labeled nucleotides. The washed E. coli cells described above (100 µl) were added to 100 µl of potassium phosphate (50 mM, pH 7.5) containing $alpha$ -³²P-labeled nucleotides (80 to 200 µCi/mmol). $alpha$ -³²P-labeled nucleoside triphosphates (NTPs) were purchased fromNEN (Bad Homburg, Germany); synthesis of [ $alpha$ -³²P]ADP from [ $alpha$ -³²P]ATP and analysis of purity were carried out as described previously(27).

Uptake of nucleotides was carried out at 30°C and stopped at the indicated time by transfer of the cells onto a 0.45-µm-pore-sizefilter (25-mm diameter; Schleicher and Schüll, Hannover, Germany)previously exposed to potassium phosphate (50 mM, pH 7.5) andset under vacuum (31). The bacterial cells were washed twicewith 1 ml of ice-cold potassium phosphate (50 mM, pH 7.5) to removeextracellular radioactivity. The filters were transferred intoa 20-ml scintillation vial containing 5 ml of water, and radioactivitywas quantified as Cerenkov radiation in a Canberra-Packard Tricarb-2500counter (Canberra-Packard, Frankfurt, Germany). All data representmeans of at least three independent experiments; the standarddeviation was always less than 8% of themean.

For back-exchange (efflux) experiments, the washed E. coli cells were preincubated at 30°C in potassium phosphate (50 mM,pH 7.5) containing 25 µM [ $alpha$ -³²P]NTP (specific activity, 1 to 2 mCi/mmol). Uptake was stoppedby centrifugation, and the sediment was resuspended in 1 ml ofpotassium phosphate (50 mM, pH 7.5) containing the indicated additions.The radioactivity in the cells was determined as describedabove.

Thin-layer chromatography of radioactively labeled guanosine nucleotides. Polyethyleneamine-cellulose thin-layer chromatography was used to identify the chemical nature of the radioactivity accumulatedby E. coli when incubated with GTP (13). Separation was carriedout for 0.5 min with 0.5 M sodium formate (pH 3.4) and 2 min with2 M sodium formate (pH 3.4), and the front was allowed to runfor 15 cm with 4 M sodium formate (pH 3.4). R_f values of radioactivelylabeled nucleotides were determined after autoradiography andcorresponded to R_f values of authentic standards visualized underUV light (13).

Nucleotide sequence accession numbers. The amino acid sequences of Npt1_Ct, Npt2_Ct, and RpTLC are available under EMBL database accession no. AJ010586, AJ010587,and M28816,respectively.

	RESULTS

Top Abstract Introduction Materials and methods Results Discussion References

Sequence and hydropathy analysis of Npt1_Ct and Npt2_Ct. The genome of C. trachomatis contains two genes, named npt1_Ct and npt2_Ct, that show significant similarity at the deducedamino acid level to RpTLC. After amplification of npt1_Ct and npt2_Ct,we cloned the entire PCR products into the pBSK vector and sequencedthe inserts. The deduced amino acid sequence of npt1_Ct differedfrom the amino acid sequence determined in the C. trachomatisgenome project at position 420, where we found a Leu instead ofa Met (Fig. 1). Npt1_Ct comprised 528 amino acids and exhibited68% similarity (Genetics Computer Group PileUp program [2])to RpTLC (Fig. 1).

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FIG. 1. Alignment of predicted amino acid sequences of Npt1_Ct, Npt2_Ct, and RpTLC. Numbers indicate amino acid positions; dots mark artificial sequence gaps introduced to improve similarity between the proteins.

The deduced amino acid sequence of Npt2_Ct comprised 540 residues, showed 61.4% similarity to the RpTLC (Fig. 1), and differedfrom the genome project sequence at 10 amino acid positions. Thesechanges were as follows: 161 Val (this study) for Ile, 208 Serfor Asn, 223 Met for Val, 256 Glu for Lys, 345 Ala for Thr, 361Val for Ile, 370 Ile for Met, 506 Thr for Ala, 508 Val for Phe,and 512 Ala for Val (Fig. 1). Three independent PCR products ofnpt1_Ct and npt2_Ct have been sequenced and found to exhibit 100%identity, indicating that the differences in the amino acid sequencesfound were not due to misfunction of the Pfupolymerase.

To gain insight into the molecular structures of Npt1_Ct and Npt2_Ct, we performed a hydropathy analysis and compared the putativestructures of the chlamydial proteins with that of RpTLC. Thisanalysis was carried out by using the algorithm developed by vonHeijne (28), which attributes specifically weight to the aminoacids deep in the membrane compared to those at the phospholipid-waterinterface. Npt1_Ct and Npt2_Ct are both highly hydrophobic proteins,and their hydrophobicity profile is consistent with their having12 transmembrane domains, a topology that has been predicted forboth the rickettsial and plastidic ATP/ADP transporters. The MEMSATprogram (9) predicted RpTLC and Npt2_Ct to be 12-transmembrane-domainproteins predicted that Npt2_Ct had only 11 transmembrane domainsbecause it failed to separate domains 11 and 12. The hydropathyprofiles of all three proteins exhibited striking similarity withrespect to the alteration and length of hydrophilic and hydrophobicdomains. However, there were notable differences in that therewere extra amino acid residues in the hydrophilic loop betweenTM6 and TM7 in Npt2_Ct and a significantly longer C-terminal regionin both chlamydial transporters (Fig. 1 and 2).

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FIG. 2. Hydropathy analysis of the predicted amino acid sequences of Npt1_Ct, Npt2_Ct, and RpTLC. Hydropathy analysis was carried out as described by von Heijne (28). The values of H, which are essentially identical, have been offset to separate the plots for clarity. The predicted transmembrane domains in RpTLC are shown at the top.

Analysis of His₁₀-Npt1_Ct. We examined the transport properties of Npt1_Ct as an N-terminal His-tagged transporter fusion protein because an N-terminalhistidine extension led to higher activities of the plastidicATP/ADP transporters when expressed heterologously in E. coli(15, 27) and a histidine tag should allow purification ofthe fusion proteins in the future. The transport of ATP and ADPcatalyzed by His₁₀-Npt1_Ct was linear for the first 2 min; afterabout 10 min of incubation, no substantial increase of radioactivityin the bacterial cells occurred (Fig. 3). In control experiments,uninduced E. coli cells did not import substantial radioactivity(Fig. 3; see also reference 27), and the activity of the unrelatedglucose 6-phosphate and glucose transport systems did not increaseafter expression of His₁₀-Npt1_Ct (data not shown; see also reference27). Increasing concentrations of exogenous [ $alpha$ -³²P]ATP or [ $alpha$ -³²P]ADP stimulated uptake to an apparent saturation at an externalconcentration of about 300 µM. A Lineweaver-Burk analysis of thedata allowed us to estimate apparent K_m values of 48 µM for ATPand 39 µM for ADP and V_max values of 370 nmol of ATP · mg of protein¹ · h¹ and 625 nmol of ADP · mg of protein¹ · h¹.

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FIG. 3. Time dependency of [ $alpha$ -³²P]ATP () and [ $alpha$ -³²P]ADP ( $open circle$ ) uptake into intact E. coli cells expressing npt1_Ct. IPTG-induced E. coli cells harboring plasmid pJT167 were incubated with 50 µM [ $alpha$ -³²P]ATP or [ $alpha$ -³²P]ADP for the indicated time periods. Control cells were not induced ( $-$ IPTG). Data are means of three independent experiments; standard deviations were less than 8% of the mean values.

The rickettsial ATP/ADP transporter operates in an exchange mode that permits the influx or efflux of ADP or ATP only whenthere is a concomitant flux in the opposite direction of ADP orATP (30). To determine if such mode of transport holds truefor Npt1_Ct transporter, we preloaded E. coli cells expressingnpt1_Ct with [ $alpha$ -³²P]ATP, removed all extracellular nucleotide, and measured thedependence of the efflux of [ $alpha$ -³²P]ATP on the presence of added unlabeled substrate in the medium.The addition of either unlabeled ATP or unlabeled ADP to the mediumto enable exchange induced a rapid efflux of 95% of the intracellularradioactivity within 5 min (Fig. 4). In contrast, medium eitherwith no additions or complemented with AMP did not support efflux,and the preloaded pool of radioactive nucleotide was retained(Fig. 4). The exchange nature of this transport system is alsosuggested by the time course of uptake (Fig. 3). Although theinflux of ADP is almost twice as fast as the ATP influx, as predictedby the kinetic values and indicated by these data, the transportof both ATP and ADP reached the same steady-state level becauseit is determined by the identical intracellular pool of ADP plusATP available for exchange.

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FIG. 4. Exchange-mediated efflux of intracellular radioactivity. IPTG-induced E. coli cells expressing npt1_Ct were preloaded by incubation with [ $alpha$ -³²P]ATP at 25 µM. After removal of external radioactivity, cells were resuspended in phosphate buffer with or without 1 mM AMP, ADP, or ATP.

To determine whether the heterologously expressed His₁₀-npt1_Ct, like RpTLC (12, 30), is specific for ATP and ADP transport,we measured the effects of related compounds on ATP uptake. Incontrast to the marked inhibition by ADP, ATP transport is onlyslightly (about 20%) inhibited by GTP, and UTP, CTP, AMP, dATP,dGTP, dCTP, and dTTP were without effect (Tables 1 and 2).

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TABLE 1. Effects of various NTPs or CCCP on transport activity of Npt1_Ct and Npt2_Ct^a

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TABLE 2. Effects of various nucleotides on transport activities of His₁₀-Npt1_Ct and His₁₀-Npt2_Ct

Analysis of nucleotide transport catalyzed by His₁₀-Npt2_Ct. Although E. coli cells expressing npt2_Ct were able to transport both [ $alpha$ -³²P]ATP and [ $alpha$ -³²P]ADP (Fig. 5A) $---$ in contrast to nucleotide transport mediated byHis₁₀-Npt1_Ct (Fig. 3) $---$ transport failed to reach a rapid steadystate and ADP uptake was substantially slower than ATP uptake.In addition, the substrate specificity of His₁₀-Npt2_Ct was muchbroader than that of His₁₀-Npt1_Ct. When GTP, UTP, and CTP wereadded as putative inhibitors at a concentration 2.5-fold higherthan that of the substrate, [ $alpha$ -³²P]ATP influx catalyzed by His₁₀-Npt2_Ct was reduced by 93, 80,and 69%, respectively (Table 1).

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FIG. 5. Time dependency of [ $alpha$ -³²P]ATP, [ $alpha$ -³²P]ADP, [ $alpha$ -³²P]GTP, [ $alpha$ -³²P]UTP, and [ $alpha$ -³²P]CTP uptake into intact E. coli cells expressing npt2_Ct. (A) Time dependency of [ $alpha$ -³²P]ATP (0.8 mM; ) or [ $alpha$ -³²P]ADP (1 mM; $open circle$ ) uptake. (B) Time dependency of [ $alpha$ -³²P]GTP (0.05 mM), [ $alpha$ -³²P]UTP (0.5 mM), and [ $alpha$ -³²P]CTP (0.5 mM) uptake.

Since the marked inhibition of ATP uptake by nucleotides other than ADP suggested that His₁₀-Npt2_Ct transported other nucleotides,we measured the transport of $alpha$ -³²P-labeled GTP, UTP, and CTP. The nucleotides were transportedby Npt2_Ct with a time course similar to that seen with ATP (Fig.5B).

The kinetic analysis revealed that GTP had the highest affinity for His₁₀-Npt2_Ct, (apparent K_m of 31 µM), ADP had the lowestaffinity (apparent K_m of about 1.8 mM), and values for UTP andCTP were intermediate (Table 3). ATP, which had a K_m of 48 µMfor Npt1_Ct, had a K_m of only 1,158 µM for this transport system.The V_max values ranged from 164 nmol · mg of protein¹ · h¹ for CTP to 109 nmol · mg of protein¹ · h¹ for GTP (Table 3).

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TABLE 3. K_m and V_max values of Npt2_Ct for various nucleotides

The inhibition by rNTPs at concentrations 2.5-fold higher than the substrate concentration affected the uptake of [ $alpha$ -³²P]GTP, [ $alpha$ -³²P]UTP, and [ $alpha$ -³²P]CTP, as predicted by the kinetics of competitive inhibitionif we assume that the K_i of a nucleotide was equal to the K_m ofthe same nucleotide. ATP, UTP, and CTP at a 2.5-fold excess over[ $alpha$ -³²P]GTP did not affect [ $alpha$ -³²P]GTP uptake substantially. [ $alpha$ -³²P]UTP uptake was inhibited strongly by GTP (4% residual activity)and to lesser extents by CTP (46% residual activity) and ATP (58%residual activity). [ $alpha$ -³²P]CTP import was inhibited strongly by GTP (8% residual activity)and to lesser extents by UTP (38% residual activity) and ATP (68%residual activity) (Table 1). As demonstrated for His₁₀-Npt1_Ct,His₁₀-Npt2_Ct was not substantially affected by dNTPs and GTP uptakecatalyzed by His₁₀-Npt2_Ct was specific for the triphosphate, sinceGMP, GDP, and guanosine tetraphosphate did not inhibit transport(Table 2).

As described above, His₁₀-Npt1_Ct catalyzed ATP/ADP exchange (Fig. 4). In contrast, His₁₀-Npt2_Ct is not able to exchange internalnucleotides with exogenously supplied nucleotides. We demonstratedthat npt2_Ct-expressing E. coli cells preloaded with either [ $alpha$ -³²P]ATP or [ $alpha$ -³²P]GTP do not release radioactivity into the medium after additionof unlabeled ATP, GTP, UTP, or CTP (data notshown).

Effect of CCCP on NTP uptake mediated by His₁₀-Npt2_Ct. Several transport systems in bacteria are energized by the symport of H⁺ driven by the proton motive force. The uptake of all four $alpha$ -³²P-labeled rNTPs by E. coli cells expressing npt2_Ct was markedlyinhibited by the protonophore m-chlorocarbonyl cyanide phenyl/hydrazone(CCCP) (Table 1). In contrast, the exchange transport catalyzedby His₁₀-Npt1_Ct was only slightly inhibited. The uptake of [ $alpha$ -³²P]GTP, the substrate for which His₁₀-Npt2_Ct exhibited the highestaffinity, was 86% inhibited by CCCP (Table 1). Based on cellwater determinations in E. coli (33), the intracellular concentrationof GTP achieved at steady state in the experiment shown in Fig.5B is approximately 1.8 mM. This represents a 36-fold (1.8/0.05)concentration gradient, of which 86% can be inhibited by CCCP.The lack of complete inhibition (in which the intracellular concentrationequals the extracellular concentration) is most likely due tobound GTP and distribution of radioactivity into compounds otherthan NTPs. This interpretation was supported by analysis of theintracellular pool after uptake of [ $alpha$ -³²P]GTP by thin-layer chromatography and autoradiography, whichwas demonstrated that about 80% of the extractable radioactivitywas transportable [ $alpha$ -³²P]GTP and 20% was nontransportable [ $alpha$ -³²P]GDP (data notshown).

	DISCUSSION

Top Abstract Introduction Materials and methods Results Discussion References

During the course of the C. trachomatis genome program, two putative ATP/ADP transporter proteins (herein called Npt1_Ct andNpt2_Ct) have been sequenced. In this study, we demonstrated thatNpt1_Ct and Npt2_Ct catalyze nucleotide transport, but of very differentsorts. There are obvious similarities in the amino acid sequencesand the hydropathy profiles of Npt1_Ct, Npt2_Ct, and RpTLC. Npt1_Ctand Npt2_Ct exhibit 68 and 61% similarity to RpTLC (Fig. 1), comparableto the similarities between the two plastidic ATP/ADP transportersfrom A. thaliana and the rickettsial homologue (10, 15). npt1_Ctand npt2_Ct generated by PCR from genomic DNA exhibited few, buthighly reproducible, differences in the deduced amino acid sequencescompared to the sequences published by the C. trachomatis genomeprogram. The differences are most likely due to the differencein serovars of C. trachomatis used for the genome analysis (serovarD) and for the experiments described here (serovarL2).

Hydropathy analysis revealed that both chlamydial proteins belong to the family of membrane-bound carriers exhibiting 12 transmembranedomains (Fig. 2), although they have no similarity in amino acidsequence to other members of this family (14). This configurationseem to represent a general feature of all nonmitochondrial nucleotidetransporters analysed so far, although in a few cases 11 transmembranedomain models cannot be eliminated. The topological arrangementof the nonmitochondrial nucleotide transporters resembles thoseof most secondary carriers, which are constructed of 12 transmembranedomains irrespective of the substrates transported or the modeof transport (uniport, symport, or antiport) catalyzed (11).The main topological differences between the chlamydial and rickettsialtransporter are significant C-terminal extensions in the chlamydialtransporters, the extra amino acids in Npt2_Ct, and the eliminationin Npt1_Ct of transmembrane domain 12 by the MEMSAT program (Fig.1 and 2). Although small truncations at the C-terminal end ofRpTLC resulted in drastically reduced transports rates (34)and a 10-his extension on the rickettsial C terminus did not interferewith activity (1), it remains to be established whether theC-terminal extensions of the chlamydial transporters influencetheir transportproperties.

His₁₀-Npt1_Ct catalyzed ATP and ADP transport when expressed heterologously in E. coli (Fig. 3). The apparent affinities forthe two compounds, K_ms of 48 and 39 µM, respectively, are similarto the adenylate affinities of RpTLC (K_m for ATP, 75 µM [29]or 100 µM [3]; K_m for ADP, 50 µM [18a]). Hatch et al. (8)estimated in C. psittaci cells K_m values for ATP and ADP of approximately5 µM. The reason for this large difference is notknown.

The observations that [ $alpha$ -³²P]ATP uptake was strongly inhibited by ADP and that external ADP or ATP promoted efflux of preloaded[ $alpha$ -³²P]ATP (Fig. 4) support the conclusions that the two compoundsare transported by the same transport protein (namely, Npt1_Ct)and that both metabolites move across the cytoplasm membrane inan exchange mode of transport. These conclusions are consistentwith the biochemical properties of the rickettsial ATP/ADP transporterand the plastidic homologues in A. thaliana (12, 15, 18,27, 30), as well as with findings for C. psittaci cells (8).

The physiological functions of the plastidic and rickettsial ATP/ADP exchange systems are obvious. For example, heterotrophicplastids are unable to synthesize ATP at sufficient rates andmust import ATP for anabolic reactions to proceed (4). BothC. trachomatis and R. prowazekii are obligate intracellular bacterialparasites that exploit the host cells for both nutrients and energy.While rickettsiae exhibit both oxidative phosphorylation and theability to transport ATP, the apparent absence of both oxidativeactivity and an electron chain in chlamydiae supported the assumptionthat these bacteria are energy parasites (16) and thus requirean ATP/ADP exchange to satisfy their energy needs. Informationobtained in the genome project suggests that, in fact, chlamydiaemay have the ability to regenerate their own ATP. Thus, most likelythe exchange of host cell ATP for bacterial ADP is an alternativemechanism to acquire energy in both organisms. In C. trachomatis,this transport is obviously mediated by Npt1_Ct. After infectionof eukaryotic cells with chlamydiae, the rate of glucose consumptionis strongly increased and a concomitant increase of the ATP concentrationoccurs (19). Assuming that the inclusion membrane that surroundsthe parasites is permeable to ATP, perhaps this facilitates theprovision of the bacterial parasite with ATP. It is worth mentioningthat little is known about transport across the inclusion membrane(6, 17).

Although Npt2_Ct exhibits remarkable structural and topological similarities to both Npt1_Ct and RpTLC (Fig. 1 and 2), Npt2_Ctpossesses totally different biochemical properties. Npt2_Ct exhibitedno substantial affinity for ADP, moderate affinity for ATP, UTP,and CTP, and very high affinity for GTP (Table 3). Npt2_Ct doesnot mediate an exchange of NTPs (as catalyzed by Npt1_Ct); rather,nucleotides accumulate in an energy-coupled manner inside thecell. For GTP, an approximately 30-fold gradient was mediatedby this transporter. The inhibitory effect of CCCP on Npt2_Ct-mediateduptake of NTPs (Table 1) indicated that NTPs enter the bacterialcells in an H⁺-cotransport mode. Such a mode of transport depends ultimatelyon the presence of a proton motive force across the parasiticcytoplasmic membrane. Indeed, it has been shown that such a forceexists in obligate intracellular bacteria (35) and supportsthe accumulation of lysine (8, 23). The stoichiometry betweenproton and NTP cotransport is unknown but must be large, sinceGTP is assumed to be tetravalent in the cytoplasm. If the stoichiometryis 4, then the transported complex is neutral and the drivingforce is $Delta$ pH and is independent of $Delta$ $psi$ . Interestingly, with thehigh stoichiometry of 4, a $Delta$ pH of 0.37 is adequate to supporta 30-fold gradient of tetravalent GTP. If the stoichiometry is3, then the transported complex is negative and a $Delta$ pH of 1.2 wouldbe necessary to obtain this gradient of GTP even assuming a modest $Delta$ $psi$ of $-$ 120 mV (the situation would become worse as $Delta$ $psi$ increased).If the stoichiometry is 5, then the complex is positively chargedand no $Delta$ pH would be needed, and a $Delta$ $psi$ of 89 mV would suffice asa drivingforce.

But what is the physiological reason for a second type of nucleotide transport system mediating net influx of molecules? GTP,ATP, UTP, and CTP are required for RNA synthesis, the formationof lipids and carbohydrate-activated intermediates, protein synthesis,and signalling. However, C. trachomatis is auxotrophic for allNTPs except CTP, which can be derived from UTP (26). Therefore,RNA synthesis, and other processes, in C. trachomatis dependsstrictly on the exogenous provision of the bacterium with NTPs,in agreement with data for C. psittaci cells (7, 25).

It is remarkable that transport proteins with a high degree of structural similarity exhibit a totally different mode of transport.Npt1_Ct catalyzes an exchange mode of transport with high substratespecificity for ATP and ADP, whereas Npt2_Ct exhibits high substratespecificity toward GTP and other NTPs and is energized by theproton motive force. Keeping these differences in mind, how greatdo the molecular differences between two proteins have to be toallow significant changes in substrate specificity or mode ofcatalysis? There are examples indicating that comparable smallchanges in the molecular architecture suffice to alter such fundamentalbiochemical properties. For example, the exchange of only twoamino acids in the strict NAD-specific leucine dehydrogenase fromThermoactinomyces intermedius leads to an enzyme which stronglyprefers NADP as a coenzyme (5). Moreover, the chemical modificationof four cysteine residues in the mitochondrial ADP/ATP carrierby application of thiol reagents alters the mode of transportfrom obligate exchange to uniport without loss of the maximalcatalytic activity (2a). It will be interesting to study thestructure-function relationships in more detail by generatingsite-directed mutants and chimeric proteins of Npt1_Ct and Npt2_Ct.

	ACKNOWLEDGMENTS

H.E.N. thanks Renate Scheibe (University of Osnabrück) for support of thiswork.

This work was financially supported by the Deutsche Forschungsgemeinschaft (SFB 171-C16). C.S. is the recipient of a graduatestudent fellowship from the Federal State Niedersachsen. Workin the lab of H.H.W. was financially supported by Public HealthService grant AI-15035 from the National Institute of Allergyand InfectiousDiseases.

	FOOTNOTES

^* Corresponding author. Mailing address: Pflanzenphysiologie, Universität Osnabrück, Barbarastr. 11, D-49069 Osnabrück, Germany.Phone: 541-9692281. Fax: 541-9692265. E-mail: Neuhaus{at}biologie.Uni-Osnabrueck.de.

REFERENCES

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

1. Alexeyen, M., and H. H. Winkler. Unpublished data.

2. Devereux, J., P. Haeberli, and O. Smithies. 1984. A comprehensive set of sequence analysis programs for the VAX. Nucleic Acids Res. 12:387-395.

2a. Dierks, T., A. Salentin, C. Heberger, and R. Krämer. 1990. The mitochondrial asparate/glutamate and ADP-ATP carrier switch from obligate counterexchange to unidirectional transport after modification by SH-reagents. Biochim. Biophys. Acta 1028:268-280[Medline].

3. Dunbar, S. A., and H. H. Winkler. 1997. Increased and controlled expression of the Rickettsia prowazekii ATP/ADP translocase and analysis of cysteine-less mutant translocase. Microbiology 143:3661-3669[Abstract/Free Full Text].

4. Emes, M. J., and H. E. Neuhaus. 1998. Metabolism and transport in non-photo-synthetic plastids. J. Exp. Bot. 48:1995-2005.

5. Galkin, A., L. Kulakova, T. Ohshima, N. Esaki, and K. Soda. 1997. Construction of a new leucine dehydrogenase with preferred specificity for NADP⁺ by site-directed mutagenesis of the strictly NAD⁺ specific enzyme. Protein Eng. 10:687-690[Abstract/Free Full Text].

6. Hackstadt, T., E. R. Fischer, M. A. Scidmore, D. D. Rockey, and R. A. Heinzen. 1997. Origins and functions of the chlamydial inclusion. Trends Microbiol. 5:288-293[Medline].

7. Hatch, T. P. 1975. Utilization of L-cell nucleoside triphosphates by Chlamydia psittaci for ribonucleic acid synthesis. J. Bacteriol. 122:393-400[Abstract/Free Full Text].

8. Hatch, T. P., E. Al-Hossainy, and J. A. Silverman. 1982. Adenine nucleotide and lysine transport in Chlamydia psittaci. J. Bacteriol. 150:662-670[Abstract/Free Full Text].

9. Jones, D. T., W. R. Taylor, and J. M. Thornton. 1994. A model recognition approach to the prediction of all-helical membrane proteins structure and topology. Biochemistry 33:3038-3049[Medline].

10. Kampfenkel, K., T. Möhlmann, O. Batz, M. van Montagu, D. Inzé, and H. E. Neuhaus. 1995. Molecular characterization of an Arabidopsis thaliana cDNA encoding a novel putative adenylate translocator of higher plants. FEBS Lett. 374:351-355[Medline].

11. Krämer, R. 1994. Functional principles of solute transport systems: concepts and perspectives. Biochim. Biophys. Acta 1185:1-34[Medline].

12. Krause, D. C., H. H. Winkler, and D. O. Wood. 1985. Cloning and expression of the Rickettsia prowazekii ADP/ATP translocator in Escherichia coli. Proc. Natl. Acad. Sci. USA 82:3015-3019[Abstract/Free Full Text].

13. Mangold, H. K. 1967. Nucleinsäuren und Nucleotide, p. 749-769. In E. Stahl (ed.), Dünnschicht-Chromatographie. Ein Laboratoriumshandbuch. Springer-Verlag, Heidelberg, Germany.

14. Marger, M. D., and M. H. Saier. 1993. A major superfamily of transmembrane facilitators that catalyse uniport, symport and antiport. Trends Biol. Sci. 18:13-20.

15. Möhlmann, T., J. Tjaden, C. Schwöppe, H. H. Winkler, K. H. Kampfenkel, and H. E. Neuhaus. 1998. Occurrence of two plastidic ATP/ADP transporters in Arabidopsis thaliana: molecular characterisation and comparative structural analysis of homologous ATP/ADP translocators from plastids and Rickettsia prowazekii. Eur. J. Biochem. 252:353-359[Medline].

16. Moulder, J. M. 1962. The biochemistry of intracellular parasitism. The University of Chicago Press, Chicago, Ill.

17. Moulder, J. M. 1991. Interaction of chlamydiae and host cells in vitro. Microbiol. Rev. 55:143-190[Abstract/Free Full Text].

18. Neuhaus, H. E., E. Thom, T. Möhlmann, M. Steup, and K. Kampfenkel. 1997. Characterization of a novel ATP/ADP transporter from Arabidopsis thaliana L. Plant J. 11:73-82[Medline].

18a. Neuhaus, H. E., and H. H. Winkler. Unpublished data.

19. Ojcius, D. M., H. Degani, J. Mispelter, and L. Dautryvarsat. 1998. Enhancement of ATP levels and glucose metabolism during an infection by Chlamydia $---$ NMR studies of living cells. J. Biol. Chem. 273:7052-7058[Abstract/Free Full Text].

20. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

21. Sarow, I., and Y. Becker. 1969. Trachoma agent DNA. J. Mol. Biol. 42:581-589[Medline].

22. Sinai, A. P., and K. A. Joiner. 1997. Safe haven: the cell biology of nonfusogenic pathogen vacuoles. Annu. Rev. Microbiol. 51:415-462[Medline].

23. Smith, D. K., and H. H. Winkler. 1977. Characterization of a lysine-specific active transport system in Rickettsia prowazekii. J. Bacteriol. 129:1349-1355[Abstract/Free Full Text].

24. Stephens, R. S., S. Kalman, C. Lammel, J. Fan, R. Marathe, L. Aravind, W. Mitchell, L. Olinger, R. L. Tatusol, Q. Zhao, E. V. Koonin, and R. W. Davis. 1998. Genome sequence of an obligate intracellular pathogen of humans: Chlamydia trachomatis. Science 282:754-759[Abstract/Free Full Text].

25. Tamura, A. 1967. Studies on RNA synthetic enzymes associated with meningo-pneumonitis virus. Ann. Rep. Inst. Virus Res. Kyoto Univ. 10:26-36.

26. Tipples, G., and G. McClarty. 1993. The obligate intracellular bacterium Chlamydia trachomatis is auxotrophic for three of the four ribonucleoside triphosphates. Mol. Microbiol. 8:1105-1114[Medline].

27. Tjaden, J., C. Schwöppe, T. Möhlmann, and H. E. Neuhaus. 1998. Expression of the plastidic ATP/ADP transporter gene in Escherichia coli lead to the presence of a functional adenine nucleotide transport system in the bacterial cytoplasmic membrane. J. Biol. Chem. 273:9630-9636[Abstract/Free Full Text].

28. von Heijne, G. 1992. Membrane protein structure prediction. Hydrophobicity analysis and the positive-inside rule. J. Mol. Biol. 22:487-494.

29. Williamson, L. R., G. V. Plano, H. H. Winkler, D. C. Krause, and D. O. Wood. 1989. Nucleotide sequence of the Rickettsia prowazekii ATP/ADP translocase-encoding gene. Gene 80:269-278[Medline].

30. Winkler, H. H. 1976. Rickettsial permeability: an ADP-ATP transport system. J. Biol. Chem. 251:389-396[Abstract/Free Full Text].

31. Winkler, H. H. 1986. Membrane transport in Rickettsia. Methods Enzymol. 125:253-259[Medline].

32. Winkler, H. H. 1990. Rickettsia species (as organisms). Annu. Rev. Microbiol. 44:131-153[Medline].

33. Winkler, H. H., and T. H. Wilson. 1966. The role of energy coupling in the transport of $beta$ -galactosides by E. coli. J. Biol. Chem. 241:2200-2211[Abstract/Free Full Text].

34. Winkler, H. H., and Y. Zhang. Unpublished data.

35. Zahorchak, R. J., and H. H. Winkler. 1983. Transmembrane electrical potential in Rickettsia prowazekii and its relationship to lysine transport. J. Bacteriol. 153:665-671[Abstract/Free Full Text].

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1.	Alexeyen, M., and H. H. Winkler. Unpublished data.
2.	Devereux, J., P. Haeberli, and O. Smithies. 1984. A comprehensive set of sequence analysis programs for the VAX. Nucleic Acids Res. 12:387-395.
2a.	Dierks, T., A. Salentin, C. Heberger, and R. Krämer. 1990. The mitochondrial asparate/glutamate and ADP-ATP carrier switch from obligate counterexchange to unidirectional transport after modification by SH-reagents. Biochim. Biophys. Acta 1028:268-280[Medline].
3.	Dunbar, S. A., and H. H. Winkler. 1997. Increased and controlled expression of the Rickettsia prowazekii ATP/ADP translocase and analysis of cysteine-less mutant translocase. Microbiology 143:3661-3669[Abstract/Free Full Text].
4.	Emes, M. J., and H. E. Neuhaus. 1998. Metabolism and transport in non-photo-synthetic plastids. J. Exp. Bot. 48:1995-2005.
5.	Galkin, A., L. Kulakova, T. Ohshima, N. Esaki, and K. Soda. 1997. Construction of a new leucine dehydrogenase with preferred specificity for NADP⁺ by site-directed mutagenesis of the strictly NAD⁺ specific enzyme. Protein Eng. 10:687-690[Abstract/Free Full Text].
6.	Hackstadt, T., E. R. Fischer, M. A. Scidmore, D. D. Rockey, and R. A. Heinzen. 1997. Origins and functions of the chlamydial inclusion. Trends Microbiol. 5:288-293[Medline].
7.	Hatch, T. P. 1975. Utilization of L-cell nucleoside triphosphates by Chlamydia psittaci for ribonucleic acid synthesis. J. Bacteriol. 122:393-400[Abstract/Free Full Text].
8.	Hatch, T. P., E. Al-Hossainy, and J. A. Silverman. 1982. Adenine nucleotide and lysine transport in Chlamydia psittaci. J. Bacteriol. 150:662-670[Abstract/Free Full Text].
9.	Jones, D. T., W. R. Taylor, and J. M. Thornton. 1994. A model recognition approach to the prediction of all-helical membrane proteins structure and topology. Biochemistry 33:3038-3049[Medline].
10.	Kampfenkel, K., T. Möhlmann, O. Batz, M. van Montagu, D. Inzé, and H. E. Neuhaus. 1995. Molecular characterization of an Arabidopsis thaliana cDNA encoding a novel putative adenylate translocator of higher plants. FEBS Lett. 374:351-355[Medline].
11.	Krämer, R. 1994. Functional principles of solute transport systems: concepts and perspectives. Biochim. Biophys. Acta 1185:1-34[Medline].
12.	Krause, D. C., H. H. Winkler, and D. O. Wood. 1985. Cloning and expression of the Rickettsia prowazekii ADP/ATP translocator in Escherichia coli. Proc. Natl. Acad. Sci. USA 82:3015-3019[Abstract/Free Full Text].
13.	Mangold, H. K. 1967. Nucleinsäuren und Nucleotide, p. 749-769. In E. Stahl (ed.), Dünnschicht-Chromatographie. Ein Laboratoriumshandbuch. Springer-Verlag, Heidelberg, Germany.
14.	Marger, M. D., and M. H. Saier. 1993. A major superfamily of transmembrane facilitators that catalyse uniport, symport and antiport. Trends Biol. Sci. 18:13-20.
15.	Möhlmann, T., J. Tjaden, C. Schwöppe, H. H. Winkler, K. H. Kampfenkel, and H. E. Neuhaus. 1998. Occurrence of two plastidic ATP/ADP transporters in Arabidopsis thaliana: molecular characterisation and comparative structural analysis of homologous ATP/ADP translocators from plastids and Rickettsia prowazekii. Eur. J. Biochem. 252:353-359[Medline].
16.	Moulder, J. M. 1962. The biochemistry of intracellular parasitism. The University of Chicago Press, Chicago, Ill.
17.	Moulder, J. M. 1991. Interaction of chlamydiae and host cells in vitro. Microbiol. Rev. 55:143-190[Abstract/Free Full Text].
18.	Neuhaus, H. E., E. Thom, T. Möhlmann, M. Steup, and K. Kampfenkel. 1997. Characterization of a novel ATP/ADP transporter from Arabidopsis thaliana L. Plant J. 11:73-82[Medline].
18a.	Neuhaus, H. E., and H. H. Winkler. Unpublished data.
19.	Ojcius, D. M., H. Degani, J. Mispelter, and L. Dautryvarsat. 1998. Enhancement of ATP levels and glucose metabolism during an infection by Chlamydia $---$ NMR studies of living cells. J. Biol. Chem. 273:7052-7058[Abstract/Free Full Text].
20.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
21.	Sarow, I., and Y. Becker. 1969. Trachoma agent DNA. J. Mol. Biol. 42:581-589[Medline].
22.	Sinai, A. P., and K. A. Joiner. 1997. Safe haven: the cell biology of nonfusogenic pathogen vacuoles. Annu. Rev. Microbiol. 51:415-462[Medline].
23.	Smith, D. K., and H. H. Winkler. 1977. Characterization of a lysine-specific active transport system in Rickettsia prowazekii. J. Bacteriol. 129:1349-1355[Abstract/Free Full Text].
24.	Stephens, R. S., S. Kalman, C. Lammel, J. Fan, R. Marathe, L. Aravind, W. Mitchell, L. Olinger, R. L. Tatusol, Q. Zhao, E. V. Koonin, and R. W. Davis. 1998. Genome sequence of an obligate intracellular pathogen of humans: Chlamydia trachomatis. Science 282:754-759[Abstract/Free Full Text].
25.	Tamura, A. 1967. Studies on RNA synthetic enzymes associated with meningo-pneumonitis virus. Ann. Rep. Inst. Virus Res. Kyoto Univ. 10:26-36.
26.	Tipples, G., and G. McClarty. 1993. The obligate intracellular bacterium Chlamydia trachomatis is auxotrophic for three of the four ribonucleoside triphosphates. Mol. Microbiol. 8:1105-1114[Medline].
27.	Tjaden, J., C. Schwöppe, T. Möhlmann, and H. E. Neuhaus. 1998. Expression of the plastidic ATP/ADP transporter gene in Escherichia coli lead to the presence of a functional adenine nucleotide transport system in the bacterial cytoplasmic membrane. J. Biol. Chem. 273:9630-9636[Abstract/Free Full Text].
28.	von Heijne, G. 1992. Membrane protein structure prediction. Hydrophobicity analysis and the positive-inside rule. J. Mol. Biol. 22:487-494.
29.	Williamson, L. R., G. V. Plano, H. H. Winkler, D. C. Krause, and D. O. Wood. 1989. Nucleotide sequence of the Rickettsia prowazekii ATP/ADP translocase-encoding gene. Gene 80:269-278[Medline].
30.	Winkler, H. H. 1976. Rickettsial permeability: an ADP-ATP transport system. J. Biol. Chem. 251:389-396[Abstract/Free Full Text].
31.	Winkler, H. H. 1986. Membrane transport in Rickettsia. Methods Enzymol. 125:253-259[Medline].
32.	Winkler, H. H. 1990. Rickettsia species (as organisms). Annu. Rev. Microbiol. 44:131-153[Medline].
33.	Winkler, H. H., and T. H. Wilson. 1966. The role of energy coupling in the transport of $beta$ -galactosides by E. coli. J. Biol. Chem. 241:2200-2211[Abstract/Free Full Text].
34.	Winkler, H. H., and Y. Zhang. Unpublished data.
35.	Zahorchak, R. J., and H. H. Winkler. 1983. Transmembrane electrical potential in Rickettsia prowazekii and its relationship to lysine transport. J. Bacteriol. 153:665-671[Abstract/Free Full Text].