Tm Jom OF BIOU~~ICAL Cmm.m~ 0 19% by Ths American Society for Biochemistry and Molaeular Biology, lnc Vol. 269, No. 9, Iisue of March 4, pp. 6290-6295, 1994 Printed in USA. Genetically Altered Levels of Inorganic Polyphosphate in Escherichia coli* (Received for publication, October 18, 1993, and in revised form, December 13, 1993) Elliott Crookes, Masahiro AkiyamaP, Narayana N. Rao, and Arthur Kornberg From the Department of Biochemistry, Stanford University School of Medicine, Stanford, California 94305 The ppk gene encoding polyphosphate kinase (PPK), the enzyme in Escherichia coli that makes long chains of polyphosphate (polyp) reversibly from ATP, was dis- rupted by insertion of a kanamycin resistance gene. Ex- pression of the exopolyphosphatase gene (ppr) immedi- ately downstream of ppk in the operon was likewise disrupted. Cells were also transformed with a high- copy-number plasmid bearing ppk. Genetically altered polyp levels were estimated in cell extracts by the PPK conversion of ADP to ATP. Polyp levels (&loll cells) near 2.0 were reduced in the ppk--ppr mutants to 0.18 and increased more than 100-fold (e.g. 220) in cells trans- formed with multiple copies of ppk. Mutant cells, lack- ing the long polyp chains, showed a growth lag following dilution of a stationary-phase culture. Polyp-deficient cells exhibit a striking phenotype in their failure to sur- vive in stationary phase and loss of resistance to heat (Sa "C) and to oxidants (42 m~ Hp02). High polyp levela are ale0 associated with reduced survival. Inorganic polyphosphate (polyp),' a long linear polymer of orthophosphates linked by high energy phosphoanhydride bonds, is widely distributed in bacteria, fungi, protozoa, plants, and mammals (1-3). Yet little is known about its cellular func- tions. Potential roles include: (i) energy source (1, 21, (ii) phos- phate reservoir (l), (iii) donor for sugar and adenylate kinases (449, (iv) chelator for divalent cations (7, 8), (v) buffer for alkaline stress (9), (vi) regulator of transcription,2 and (vii) component in competence for DNA entry and transformation (10). A membrane-associated enzyme in Escherichia coli, poly- phosphate kinase (PPK), catalyzes the synthesis of polyp from the terminal phosphate of ATP in a freely reversible reaction (nATP ++ nADP + poly€',) (11-13). Cloning of theppk gene (14) also identified an adjacent gene, ppx, which encodes an exo- polyphosphatase (PPX), an enzyme which processively releases orthophosphate from the termini of polyp in the reaction (polyp, -+ polyPn-l + Pi) (15). Expression of ppr is dependent upon the ppk promoter, indicative of a polyphosphate operon (15). * This work was supported in part by granta from the National In- stitutes of Health and the National Science Foundation (to A. K.). The coats of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked hduer- tisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact. $ Supported by American Cancer Society, California Division Senior Postdoctoral Fellowship S-26-91. F'reaent address: Dept. of Biochemb- try and Molecular Biology, Georgetown University Medical Center, Washinen, D. C. 20007. I Present address: Cold Spring Harbor Laboratory, Cold Spring Har- ~~ bor, NY 11724. 1 The abbreviations used are: polyp, polyphosphatc PPK, polyphos- phate kinase; PPX, exopolyphosphatase; MOPS, 4-morpholinepropane- sulfonic acid; kb, kilobaae pair(s). 2 A. Ishihama, personal communication. In attempts to elucidate the functions of polyp, we have con- structed mutants that fail to express ppk and ppx as well as cells which overproduce PPK. The consequences of altering the level of polyp 1,000-fold have been examined. MATERIALS AND METHODS Reagents-Sources were: ATP, ADP, creatine kinase, DNase I, and RNase IIIa, Boehringer Mannheim; creatine phosphate, MOPS, and polyp glass (type 65), Sigma; [(r-aaPldATP and [yS2PlATP, Amersham Corp.; restriction endonucleases. New England Biolabs; Immobilon-N membrane, Millipore; and polyethyleneimine-celluloae F thin-layer chromatography plates, Merck. Bacterial Strains, Plasmids, and Phages-E. coli K12 derivatives were: DH5o (F, supE44, A~lacZYA-argF)Ul69[+801acZAMl51, hadRl7, reCA1, endAl.gyrA96, thi-1, relAI, &OR); SC864 (P, polA12(ts), thi-1, thr-1, leuBG,lacYl, fhuA21, supE44, fod751::TnlO. A-); JMlOl (Allac- proAB), supE, thi-lP'ftraD36, proAB*, laclq, hcZAMl5J; CF1648 (F-, A?; NK6056 (Mgpt-lack5, purC8O:TnlO, relA1, spoT1, thi-1, A-); N3007 (A; gw-26:TnlO (in guaA or guaB), IN(rrnD-rrnE)l). DH6a was the host strain for plasmid preparations. SC864 was used to constructppk- mutants by inserting, through homologous recombination, the kan gene into ppk on the E. coli chromosome, as described below (Fig. 2). The mutated ppk genes were transferred into JMlOl by P1 transduction (16); CAlO contains the kan gene in the same orientation as ppk whereas CAll contains kan in the opposite orientation. NK6066 and N3007 were used to map the integration site of kan on the chromosome. Phage A 10H6 (14, 17) was from the Kohara A library (17). Plasmid pBC8 (Figs. 2 and 4) was used as a probe for Southern blotting. Plasmid pBC29 used for polyp overexpression is a multicopy plasmid bearing ppk (15). Survival Assays-Long-term survival ofE. coli was assayed by grow- ing cells in MOPS-buffered minimal medium (18) containing glucose (0.1%) as the carbon source and K,HPO. (2 m~) as the P, source. Cul- tures (3 ml) incubated at 37 "C for prolonged periods in glass test tubes (18 by 200 mm) were aerated by rotation in a New Brunswick gyratory wheel. Viable cell counts were determined by plating onto MOPS-buff- ered minimal agar medium containing 0.4% glucose and 2 nm &HPO,; kanamycin (50 &ml) was added to the medium on which the mutant CAlO was plated. For the heat-shock survival assay, cells were gmwn overnight (-20 h) in LB. The stationary-phase cells were washed and diluted in 0.9% NaCl to a density of about 5 x 103 celldml. Samples (2 ml) were put in glass tubes prewarmed to 55 "C and at times indicated, aliquots (0.1 ml) were plated directly on LB plates to determine viable cell numbers. To test sensitivity to HzO2, cells were grown overnight (-20 h) in LB, washed, and resuspended in 0.9% NaCl to an ODm of 1.0. HzOz wa8 added to a final concentration of 42 m~. At the times indicated, 0.1-ml samples were withdrawn, diluted immediately in 0.9% NaCl and plated onto LB plates to determine viable cell numbers. Extraction of Polyp from E. coli-LB medium (1,500 ml) was inocu- lated to an optical density (Asw ,,=) of 0.06 with a sample ofan overnight culture and incubated at 37 "C. Cells were harvested by centrifugation (6,000 xg, 7 min, 2 "C) when the culture reached mid-log phase growth. The resulting cell pellet was resuspended and lysed in ice-cold 2% trichloroacetic acid (0.6 ml); the suspension was maintained at 0 "C for 30 min with occasional vigorous mixing. Acid-insoluble material was collected by centrihgation (3 min, 14,000 x g. 2 "C), and the pellet was washed with ice-cold 67% acetone (1 ml) and collected by centrifugation, as above. The pellet was resuspended in 50 mM HEPES-KOH, pH 7.5 (0.5 ml), and the pH was adjusted to neutrality by the addition of 0.2 M KOH. MgCI, (5 m~), DNase I, and RNase IIIa (300 pdml of each) were added, and the mixture was incubated at 37 "C for 30 min. Proteinase 6290 Inorganic Polyphosphate in E. coli 6291 m i 0 VJ 0 100 200 300600 Polyp Added (pmol ol Pi) FIG. 1. Fewtic assay for polyp. Synthetic polyp glass (type 65) solutions of known concentration (aee 'Materials and Methods") were incubated with ['T-UIADP and purified PPK The level of ATP formed was determined as described (see 'Materials and Methods"). K was added (600 dml) and the incubation was continued for an additional 45 min. The mixture (approximately 1 ml) was extracted with phenolxhloroform (0.5 ml, 1:1, equilibrated with 0.1 M ammonium acetate), the phases were separated by centrifugation (5 min, 14,000 x g, room temperature), only the aqueous phase was removed and dis- carded. Additional portions of pheno1:chloroform (0.2 ml) and 50 m~ HEPES-KOH, pH 7.6 (0.6 ml), along with EDTA(to 10 m~) were added to the interfacial material and organic phase. The sample was mixed vigorously, incubated at 37 "C for 5 min, and the phases were separated by centrifugation, as above. The aqueous phase was removed and re- tained. Extraction of the organic phase was repeated three more times with 50 IIIM HEPES-KOH, pH 7.6, 10 m~ EDTA (0.25 dextraction), and all of the aqueous phases containing EDTA were pooled. The pooled sample was treated twice with water-saturated chloroform (1 ml/ extraction), followed by the addition of ice-cold sec-butanol(1.0 ml). The mixture was kept at -20 "C for 30 min or more, and the precipitated polyp was collected by centrifugation (15 min, 14,000 x g, 2 "C). The pellet was washed with ice-cold acetone (1 ml), dried under vacuum, and resuspended in water (0.2 ml). Assay for Polyp-The ability to serve as a substrate for the PPK- catalyzed conversion of ADP to ATP was used as an assay to quantitate levels of polyp. The reaction mixture (10 pl) contained: 50 m~ HEPES- (0.1 Ci/mmol), 2,000 units PPK, and polyp as indicated. The reaction (37 "C for 45 min) was terminated by chilling to 0 "C and the addition of ADP and ATP (to 5 m~ of each). Aliquota were spotted onto a poly- ethyleneimine-cellulose F thin-layer chromatography plate; polyp, ADP, and ATP were resolved using 0.4 M LiCI, 1.0 Y HCOOH a8 a solvent system and visualized with UV-irradiation. The radiolabel that re- mained at the origin and that which migrated with ADP. ATP, and the solvent front was quantitated by liquid scintillation counting. With ADP in excess, PPK catalyzed the almost complete consumption of polyp, yielding an equivalent amount of ATP (Fig. 1). Other Procedures-PPK and PPX were assayed as described (14,16). PPK (3 x 10' uniWmg) was purified as described (14). [3aP1PolyP was synthesized with PPK from [y-31PPIATP and purified (15). The concen- trations of polyp glass (type 65) solutions were determined by measur- ing total phosphate (19). KOH, PH 7.2,40 IIIM (NH&SO,, 4 m~ MgCI,, and 11.6 1°C-UIADP RESULTS Disruption of the ppk Gene-A 9-kb fragment of E. coli DNA spanning both ppk and ppx was cloned from phage blOH6 (14, 17) into the vector pBR322 (Fig. 2.4). "he EcoRI site near the middle of the fragment is approximately 0.3 kb downstream of the start codon for ppk (14). A 1.3-kb DNA fragment of plasmid pUC4K (Pharmacia LKB Biotechnology Inc.) containing the kan gene waa inserted at this EcoFtI site in either orientation relative to theppk gene to produce plasmids pBC22 and pBC24 (Fig. 2B). The wild-type ppk gene on the E. coli chromosome was re- placed with the disrupted ppk gene by exploiting the require- ment for functional DNA polymerase I to replicate plasmids with a ColEl origin. A strain (SC864) with a temperature- sensitive DNA polymerase I was transformed with pBC22 and pBC24 at a permissive temperature (30 "C). In addition to con- taining the inserted gene for kanamycin resistance, the plas- mids also confer resistance to ampicillin through their pBR322 component. During growth at the permissive temperature, plasmids may integrate into the host chromosome by recombi- nation between homologous regions of the plasmid and the chromosome (integration), or a part of the chromosome may be replaced with the corresponding cloned DNA by a double cross- over event (replacement) (Fig. 3). When such cells are shifted to the nonpermissive temperature (42 "C) for DNA polymerase I function, plasmids are lost. Only those cells with a kan gene inserted into their chromosome can survive exposure to kana- mycin. Ampicillin- and kanamycin-resistant transformants were se- lected at the permissive temperature of 30°C. Cultures of transformants were grown overnight at 30 "C in LB medium (16) containing ampicillin (50 pg/mU and kanamycin (50 pgl ml). Aliquots of each culture were used to inoculate LB medium containing kanamycin (50 &ml) for overnight growth at 42 "C. Appropriate dilutions of the cultures were spread onto LB agar plates containing kanamycin (50 pg/ml), and the plates were incubated at 42 "C. The resulting kanamycin-resistant colonies were screened for sensitivity to ampicillin. Kanamycin-resist- ant, ampicillin-sensitive cells (ppk::kan) were isolated from SC8WpBC22 and SC864IpBC24, and the disruptedppk genes were transferred to the strain JMlOl by P1 transduction yield- ing strains CAlO and CA11, respectively. Confirmation of Disrupted ppk Genes-A 4.4-kb SalI frag- ment upstream of ppk was subcloned from X10H6 into the vector pUC18, and the resulting plasmid, pBC8, was used as a probe for Southern blotting. The ppk- mutants were examined by Southern blotting (Fig. 4). The radiolabeled probe pBC8 hybridized to a 4.4-kb SalI fragment of genomic DNA from JMlOl (Fig. 44, lane I ), but not from CAlO or CAll. Instead, CAlO and CAll yielded a 5.1-kb fragment (Fig. 4A, lanes 2 and 3) as expected from examination of their physical map (Fig. 3B). The smaller band in lane 4 corresponds to vector plasmid pBR322. Since HindIII endonuclease digests the kan gene into 0.6- and 0.7-kb fragments, the orientation of the inserted kan gene relative toppk was confrmed by Southern blotting of SalI and HindIII-digested genomic DNA (Fig. 48). Whereas the 4.4-kb fragment from JMlOl was not affected by the additional digestion with HindIII (Fig. 4B, lane 1 ), the 5.1-kb fragments from CAlO and CAll were altered, confirming the insertion of the kan gene into ppk; the size difference of the resulting frag- ments demonstrates that kan is in the same transcriptional orientation asppk in CA10, whereas in the opposite orientation in CA11. Following a SaZI-Hind111 digestion, the expected 0.9-kb fragment from CAlO and 1.0-kb fragment from CAll were found to hybridize to pBC8 with a longer exposure of the gel (data not shown). Additionally, transduction frequencies with P1 phage revealed that the gene for kanamycin resistance in CAlO is closely linked to guaAB and PUS, genetic markers close to ppk (20) on the E. coli chromosome (data not shown). PPK and PPX Activities in Mutant CAlO and CAI1 Cells- Lysates prepared from JM101, CA10, and CAll cells were as- sayed for PPK and PPX activities (Table I). JMlOl cells con- tained PPK and PPX in quantities comparable with other wild- type cells (14, 15). However, in CAlO and CA11, cells in which the ppk gene has been disrupted, the levels of both PPK and PPX were below the limit of detection. Immunoblot analysis using anti-PPK serum also failed to detect PPK in the ppk- strains (Fig. 5); analysis with anti-PPX serum also confirmed 6292 Inorganic Polphosphate UL E. coli Pic, 2 Maps of phage and plasmid DNrts. .4, it rcgion of phage ~10II6 (14, 17) The Ed21 -ite 41uwn at thepnctton of the E' cofr ONA insert and the A DN.4 wine from the h DNA The thtrk line &ove thc map shoKs the 4 4-kb Sal1 fmg- ment cloned into pH pRC22 and pBC24 PI \tructed a\ dc scribed n indicate the direction d transcnption DXA fragnent len@hs are sho\rn in kilo- base patrs Symbols are ,~nfillvd hox, E tolc DXA Flkd hm apk gene, cross- itotrhed hvx, ppx gene. \tippled hox, ) kat2 gcne tragment, uav\. line, h thin Irn~, 'Icetor pBIi322 DNA Ah- Ittons arcs R, IlanrHI, E:, EmKI. N, HrndIiI S Sol1 Km' Ap' 30" c 4 30°C 58 _I 10 L- - 58-------- .. ,~ +- 1 42°C A-2 Integration Km' Ap' Replacement Km' Ape Fir, 3 Stratem for the isolation of ppk:daan mutants. Strain5 divupted for ppk expression were isolated a:: dcscnbed in thP text Sqmbols used itre fitifilied box, cloned E. colt chromosonial DNA crosrc hatched bo*. region of the E coli chromosome corresponding to the cloned DK.4, I kari gene inserted into the cloned ppk gene, thick he. haetenal chromosome, thio Irne, wctor pBR322, KmF, kanarngcln re- 5iatance Ap,, d~npicillin re an=. tip . ampicillin sens the absence of PPX (data not shown). Polyp C'oriteiii in w7ki-t.vpc CPLLS, ppk-ppx- Mufarits, rind Cells Ocwprociucrng PPK-Polyp was extracted from cells with wild-type (JM101 and JMlOYpUClHi and mutarit ICALO and C'A11) levels of PPK and PPX and with overproduced tdMlOli pBC29) 161 levels of PPK The extraction procedure separated polyP from other phosphate-containing compounds in the ccll lysate by its insolubility in cold acid and organic solvents, re- sistance to nucleases and proteases, and chelation by MgL+ (see "hlateriats and Methods"). [ '"P1PolyP, added to a portion of the initial cell lysates a5 a marker, was recovered with a yield of 90Y or geiitm The pol.yP content of extracts prepared from the banous ccll types was measured using the PPK conversion of ADP to ATP, 1 kb A B Sal I Sal 1 -Hind Ill 1234 1234 kb 8.0 _- 7.0 - 6.0 - -wm 5.0 - 4.0 -- 3.0 - I* - 4 vectoi 2.0 - 1.5 - ---I* 1.0 - 0.5 - Fib 4 Southern blot analyeis of ppk- mutant genomic DNA. E CO~L genomic DNA was prepared from the ppk* strain 1JMl01 I and the ppk- mutant strains rlcctrophoresis cB) through an agarosc gel I I"r I. traii+mcd trr an Imniobilun-N filter, and prolwd with radiolabeled pRCH DNA. Lane 1, ,JMlOl gennmtc DNA. lone 2, CAlOgenomic DNA, low 1, CAI1 gcnomlc DXA, lonc. 4, piasmtd pBCH UNA as descnhed above. Cellular polyP concentration was about 2 0 pgt10" cells in the wild type cells (JM101) and wild-type cells transformed with the vector plasmid (Table I1 I. Another E coli wild-type strain CF1648 contained 0 44 pg of cellular polyp Cells overexpressing PPK had polyp at level^ over 100-fold Inorganic Polyphosphafe in E. coli T,WI k I Strains iJM101, CAIO, and CAll I \\ere gmwn in 1,N medtum at 3; C L:i\utc>c from {~pk 5lminh lntk I'PK nr,d PP,Y a( Iitvtrr*c to an optical den3tty rA,,, %)I of 1 Cells were h tion and lysed as dcscnbed I 14,151 PPK acti5it wnicated lybate pellet fraction 1141, and f'PX a for the soluble lysate fraction (15, Activities of PPK PI% " ... ',... ~ .... "" ~ ........ . .... ,',.. Strain JMlOl CAI0 CAll UlIIf\ x 10 "E cci! <3 0 <5 3 <2 4 <3 8 320 'L!W Purilied PPK (ng) Culture (111) JMlOl CAlO 6 18 60180 50 200 800 50 200800 Mr 97 - 68 - 43 - 29 - 18 - FIG. 5. Cellular abundance of PPK. Cells cJM101, CAlOi were grown at 37 "C in LB medium to an optical density (OD, ,,ml of 1 8 Total cell protein was precipitated from 13 mi of the culture with tnchloroacetic acid ( 10"r final concentration) The precipitate -45 hdr- vested in d hlicrofuge, washed bite with 1 ml of ice-cold acetone. and solubilized in SDS-PACE buffer Samples were subjected to SDS-PAGE (15%) PPK H~S detenurned by immunoblotting with PPK antiserum Punfied PPK served as a standard T\fm I1 PolyP contr,.it of cells u zth altcrd expresaton of ppk and ppi Extracts ennched for plqP were prepated (see "Matenalb and Meth- ods") and their polvP content waii determined as for solutions of polyP glass tF1g 1) t / . CAlO I 0 2 3 Hours 6293 00 10 2C 30 40 1071 . ' - - -I ~ __ -- _I_ ' &says of Pol) P extracted from three different cultures were aver- aged higher than wild-type cells. Polyp levels in mutant cells (CAI0 and C.411) that lacked a functional ppk and ppr operon were 0.16 pgilOii cells. The extracts from these mutant cells were not inhibitory to the PPK-catalyzed production of ATP. in that a mixture of CA10 extract and synthetically prepared polyp was indistinguishable from that of polyp alone idata not shown) Preliminary analysis of the polyp from the mutant cells indicatad that they were predominantly short chain poly- mers with an average chain len@h of 60 (data not shown,. It is likely that these short chain polyp are synthesized by an inde- pendent pathway. Cells UefTcLvrit in Polyp Exhibit R Grouth Lag-\Vhen JM10S (PPK-) and CAI0 (PPK", cells were grown on minimal medium (M9 t 0 29 glucose) plates (16f, the mutant cells showed slow growth (small colony sizei during the early stages of the incu- bation (data not shown) However, with further puwth the Hours Fitl. 6 Growth of wild-type cells and mutants lacking long ehnin polyp. Cells IJ>llOl and CA10, were mown in the irtdrcated media tu saturatitin Prewarmed 137 c', media Rere inoculated wtth sdniyles of the stationary ritlturcs and incubated at 37 C Appropnatc. dilutions of tht. cultures upre plated onto mtdia to monitor &To>\ th Media werc '4, LB I 16% and B, Y9 + 0 2'1 glucosr t 161 differenct. in colony size decreased The initial growth of the two cell types was measured following the inoculation of vari- ous media with stationarq-phase cultures In a nch medium tLB), the cell number for wild-type cells started to increase after 1 h whereas the growth lag tor mutant cells %as repro- ducibly longer (Fig a), this lag wah also observed using a minimal glucose medium (Fig SH 1 Effccts of lWyP Dt.ficienr?; on Long-term Sur~it nl in Station- ary phase, 77~ermal Rrstctancr, and N.D1 Resistance--E col~ mutant strain ChlO uhich lachs PPK and PPX exhibited re- duced surtibal in btationary phase (Fig ~AJ After 2 days in stationary phase in minimal medium with limited carbon source IO 1% glucose~, the wnbility of the mutants dropped to 7': of the orignal balm (Fig 7Aj The corresponding wld- type strain (JM101 I did not show any significant loss tn v ity dunng this pertod In addition to the loss in viahilit>, a 6294 Inorganic Polyphosphate in E. coli JM101 a10 JM101 0123466 Time (mlnuteo) 0 20 40 60 BO TIme (mhutesl FIG. 7. Physiological teste. A, long-term survival of wild-type E. coli (JM101) and the polyp-deficient mutant (CA10) in MOPS-buffered minimal medium with limited glucose (0.1%. w/v). Percent survival represents the viable cell number at each time point divided by the viable cell number of the same culture after 24 h in stationary phase. Similar results were obtained in three experiments. B. heat-shock sur- vival. Cella were grown overnight (-20 h) at 37 "C in LB medium, exposed to 55 "C, and the viability determined by plating on LB agar; 100% is equivalent to -5 x lo3 celldml. C, Hz02 sensitivity; stationary phase cultures were exposed to 42 m~ Hz02, and viable cell numbers were determined as described under "Materials and Methods"; 100% corresponds to the viable cell number determined immediately before the addition of HzOz. stable small colony phenotype emerged from stationary-phase CAlO cells after 48 h in stationary phase (data not shown). During survival in stationary phase or starvation, E. coli cells acquire rpoS (kat Fkmediated resistance to multiple stresses, including heat and oxidants (25-28). When polyp-deficient cells (CA10) were held at 55 "C for 2 min, only 2% survived, as compared with about 90% of the wild type (JM101) (Fig. 7B). Similarly, of the polyp-deficient E. coli cells in stationary phase exposed to 42 mM HzOz, only 40% survived as compared with about 85% of the wild type (Fig. 70. DISCUSSION The ease with which orthophosphate condenses to form in- organic polyphosphate (polyp), a polymer linked by phospho- anhydride bonds, argues for a prominent role for the energy- rich compound in prebiotic evolution. In view of the ubiquity and abundance of polyp throughout nature, presumptions of multiple roles for this molecular fossil are reasonable, but ex- actly what these are must vary depending on where and when polyp serves in cellular functions. In our approach to identify and examine polyp functions, we have purified enzymes responsible for the synthesis and utili- zation of polyp. The homogeneous enzyme provides a route to the discovery of the gene which encodes it and a means of modulating gene expression from depletion to overproduction of the enzyme. Phenotypes created by this "reverse genetics" may supply clues to the physiologic functions of polyp in cellu- lar growth, metabolism, and development. Often unappreci- ated is the immediate utility of the purified enzyme as a rea- gent to prepare labeled well defined substrates and as an analytical tool to determine the features and abundance of polyp in extracts of various cells and organisms. Previously, we identified the E. coli genes ppk for a polyp kinase (PPK) (14) and ppx for an PPX (15). These adjacent genes form an operon, the functions of which in polyp metabo- lism needs to be explored. To this end, we have constructed the mutant strains, reported in this study, in which the expression of ppk and ppx have been disrupted (Table I); overexpression of these genes, introduced in high copy number plasmids, has been obtained (14, 15). By these manipulations, the levels of polyp have been reduced more than 10-fold in the mutants and raised about 100-fold in the overproducer (Table ID, an overall spread in the level of 1,000-fold. The mutant cells are viable and show no striking phenotype as judged by growth in various media. Rates do not differ from wild-type cells in rich media at temperatures between 23 and 42 "C, in media limited in carbon (16) or in phosphate (211, at high ionic strength (eg. 330-800 mid or at decreased oxygen tensions (22). Nor were any growth rate differences observed between wild-type, mutant, and overproducer cells in a mini- mal medium containing a nonfermentable carbon source (e.g. succinate) or in the presence of dinitrophenol or azide at levels sufficient to reduce cellular ATP. The polyp content of wild-type cells grown on succinate was also similar to that of cells grown on glucose. The most suggestive indications of a deficiency in the ppk mutant are in the adjustments made in response to nutrient deprivation and for survival in the stationary phase. Guano- sine pentaphosphate hydrolase, one of the two enzymes (the other being RelA which synthesizes pppGpp) essential for mak- ing ppGpp in response to the stringency of amino acid starva- tion (23). has unexpectedly turned out to be a potent exopoly- phosphatase, different from PPX (24). Furthermore, polyp levels increased 10-fold or more in cells treated with serine hydroximate, an amino acid analog that induces (p)ppGpp pro- d~ction.~ How polyp is involved in regulating promoter selec- tion in this and other circumstances remains to be determined. The ppk mutant is impaired in responses to stress and dep- rivation. There is a striking lability to heat and to hydrogen peroxide; survival in the stationary phase is also affected (Fig. 7). After the second day in a minimal medium with a limited carbon source at 37 "C, there is not only a greater loss of vi- ability in the mutant strain, but also the emergence of a small colony variant. These and other changes are suggestive of a selection for rpoS (katF) alleles that direct patterns of gene expression essential for adjustments to remaining viable in the stationary phase (25-28). Cells with elevated polyp levels (JMlOl/pBC29, Table 11) attained only one doubling in cell density when grown in minimal medium. The viable cell num- ber at this stage was less than 4% of the wild type at stationary phase (data not shown). Polyp has been identified as a component of a complex with polyhydroxybutyrate and Ca2+ in the membrane of bacteria competent for DNA transformation (10). The mutant strain with reduced levels of polyp can still acquire competence, al- E. Crwke and A. Kornberg, unpublished data. Inorganic Polyphosphate in E. coli 6295 though with less efficiency than the wild type.4 The competent mutant strains do possess a chloroformextractable polyp chain of about 60 residues, presumably synthesized by a pathway other than PPK.5 A remarkable ecological contribution made by PPK is in the bacterial removal of phosphate which pollutes waterways and causes algal blooms. In current sanitary engineering practice, an aerobic fermentation fixes phosphate in ATP, which is then converted by PPK to polyp and removed with the bacterial sludge (29). By transforming one of the bacterial strains with a high copy number plasmid bearing the ppk gene, phosphate removal from the surrounding medium became far more rapid and complete.6 With a similar plasmid bearing both the ppk and ppx genes, overproduction of the PPX counteracts the ef- fectiveness of PPK, a clear demonstration of the actions in vivo of each of these enzymes. Acknowledgments-We thank Dr. Stanley Cohen (Stanford Univer- sity) for Pl phage and strain SC864, Dr. Barbara Bachmann (E. coli Genetic Stock Center, Yale University) for strains NK6056 and N3007, Dr. Michael Cashel (National Institutes of Health) for strain CF1648, and Dr. Yuji Kohara (National Institute of Genetics, Japan) for the Kohara phage library. REFERENCES 1. Kulaev, I. S. (1979) The Biochemistry oflnorganic Polyphosphafes. John Wiley 2. Wwd, H. G., and Clark, J. E. (1988)Annu. Rev. Biochem. 57,235-260 3. Pisoni, A L., and Lindley, E. R. (1992) J. Biol. Chem. 287,36263631 & Sons. New York E. Crooke, C. E. 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