The C-Terminal Sequence of the lambda  Holin Constitutes a Cytoplasmic Regulatory Domain

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Journal of Bacteriology, May 1999, p. 2922-2929, Vol. 181, No. 9
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

The C-Terminal Sequence of the $lambda$ Holin Constitutes a Cytoplasmic Regulatory Domain

Udo Bläsi,¹ Peter Fraisl,¹ Chung-Yu Chang,²^, Ning Zhang,² and Ry Young²^,^*

Institute of Microbiology and Genetics, Vienna Biocenter, 1030 Vienna, Austria,¹ and Department of Biochemistry and Biophysics, Texas A&M University, College Station, Texas 77843-2128²

Received 30 November 1998/Accepted 23 February 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The C-terminal domains of holins are highly hydrophilic and contain clusters of consecutive basic and acidic residues, withthe overall net charge predicted to be positive. The C-terminaldomain of $lambda$ S was found to be cytoplasmic, as defined by proteaseaccessibility in spheroplasts and inverted membrane vesicles.C-terminal nonsense mutations were constructed in S and foundto be lysis proficient, as long as at least one basic residueis retained at the C terminus. In general, the normal intrinsicscheduling of S function is deranged, resulting in early lysis.However, the capacity of each truncated lytic allele for inhibitionby the S107 inhibitor product of S is retained. The K97am allele,when incorporated into the phage context, confers a plaque-formingdefect because its early lysis significantly reduces the burstsize. Finally, a C-terminal frameshift mutation was isolated asa suppressor of the even more severe early lysis defect of themutant SA52G, which causes lysis at or before the time when thefirst phage particle is assembled in the cell. This mutation scramblesthe C-terminal sequence of S, resulting in a predicted net chargeincrease of +4, and retards lysis by about 30 min, thus permittinga viable quantity of progeny to accumulate. Thus, the C-terminaldomain is not involved in the formation of the lethal membranelesion nor in the "dual-start" regulation conserved in lambdoidholins. Instead, the C-terminal sequence defines a cytoplasmicregulatory domain which affects the timing of lysis. Comparisonof the C-terminal sequences of within holin families suggeststhat these domains have little or no structure but act as reservoirsof charged residues that interact with the membrane to effectproper lysistiming.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Holins are small integral membrane proteins which are required for host lysis by most double-stranded DNA bacteriophage. Thebest-studied holin gene is the $lambda$ S gene, which spans only 107codons and is the first gene in the sole $lambda$ late gene transcript(6, 41, 42). Endolysins are diverse soluble bacteriolyticenzymes which accumulate in the cytoplasm of the infected cellduring the vegetative phase. Examples of endolysins are the $lambda$ gene R transglycosylase, the T7 gene 3.5 amidase, and the P22gene 19 lysozyme, enzymes with unrelated mechanisms and differentevolutionary lineages (2, 8, 11). The function of theholin is to cause the formation of membrane lesions ("holes")which allow the escape of the soluble endolysin and the subsequentdestruction of the cell wall. Equally important, the holin hasan essential timing function which causes it to form the holesat a genetically programmed time. The holin is a "clock" whichthus determines the length and productive burst size of the phageinfective cycle (41).

Nothing is known about the structure of the putative hole or the mechanism of hole formation, topics which may be fruitfullyapproached now that purified holin protein is available (34).However, substantial genetic information has been obtained regardingthe components of the timing function. The first three codonsof $lambda$ S are Met₁-Lys₂-Met₃-, and it has been established that translationalinitiations occur at both Met codons in vivo, generating two geneproducts, S107 and S105, that differ only in the first two residues.Remarkably, the two proteins have opposing functions, with S105being the active holin and S107 acting as a holin inhibitor (6).Thus, the lysis clock is set, to a significant extent, by theproportion of initiation events at the two start codons (5,10, 31). The operational difference between S107 and S105is the cationic side chain at position two in S107, and puttinga second basic residue between the two start codons makes theinhibitor form even more inhibitory (4, 28). The inhibitorycapacity of S107 depends on the energized membrane (4), leadingto the simplest model that the N-terminal positive charge of S107interacts electrostatically with the predominantly anionic innersurface of the cytoplasmic membrane. Interpretation of these factsis hampered by the absence of firm topological information regardingthe membrane topology of S, which, from inspection of its primarysequence, has three potential transmembrane domains (Fig. 1).

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FIG. 1. Features of the primary sequence of S. The predicted sequence of the $lambda$ S107 gene product is shown, with shaded bars over the three potential transmembrane domains and a hatched bar above the hydrophilic C-terminal domain characteristic of holins. Shown on the left is a blow-up of the amino-terminal sequences of the S107 and S105 products, including the corresponding mRNA sequence of the translational initiation region and the sdi stem-loop structure (31). Shown on the right is a blow-up of the C-terminal hydrophilic domain, including the corresponding mRNA sequence and, below that, the +1 frameshift mutation of $lambda$ aj1, isolated as a suppressor of the plaque-forming defect of SA52G (also shown) (21). The time of lysis onset is shown in parentheses for both the SA52G early-lysis mutant and $lambda$ aj1.

Many holin sequences have been reported since the holin-endolysin model was first formalized as a fundamental strategy forphage lysis (41, 42). Many holins apparently have the "dual-start"motif described above, although evidence for homologous functionfor the motif is available only for the holin genes of the lambdoidphage 21 and the B. subtilis phage $phi$ 29 (1, 7, 38). Aneven more universal characteristic is the existence of a C-terminalsequence which is rich in residues charged at physiological pHand usually with a significant net positive charge (41, 42)(Fig. 2). This makes it likely that the C terminus is localizedto the cytoplasm, according to the von Heijne "positive inside"rule (39). Moreover, in many cases, there are multiple chargedresidues in a sequence, including 10 residues in a row in theN15 holin sequence. In addition, in several cases, there is, withinan orthologous group of holins, at least one ortholog in whichthe C-terminal domain is completely dissimilar or in which thesequence similarity ends abruptly in the middle of the domain(Fig. 2; see P2 Y and its ortholog from phage 186, 21 S and itsortholog from $phi$ 80, and Hp1 Orf78 and its ortholog from the crypticprophage of H. somnus). Assuming the C termini of holins havea common function, it is unlikely that such changes are compatiblewith a highly structured domain but rather that this domain mayserve as a reservoir of charged residues with a function analogousto that of the N-terminal motif. If the C-terminal domain is highlycharged and largely unstructured, we reasoned that it might bepossible to effect truncations of the C terminus which left thelytic capacity of the S protein intact, although the timing functionmight be deranged. Here we report the results of a molecular andphysiological analysis of the C-terminal domain of the $lambda$ holin.These results are discussed in terms of a model for holin functionand regulation.

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FIG. 2. The C-terminal hydrophilic domain of holin proteins from bacteriophages of gram-negative bacteria. The C-terminal sequence of the first member identified from each of the orthologous groups of holins is shown. Holin sequences are grouped into class I (three potential transmembrane domains) and class II (two potential transmembrane domains). Each holin is given with the total number of residues for the longest form of the predicted protein product. Class I orthologous groups: $lambda$ S (four orthologs, including P22 gp13), N15 (no orthologs), P2 Y (one ortholog, 186 Orf24), P1 LydA (no orthologs), and PRD1 OrfM (no orthologs). Class II orthologous groups: 21 S (six orthologs, including $phi$ 80 S); Hp1 Orf78 (one ortholog, Haemophilus somnus cryptic holin), T7 gp17.5 1 ortholog, and T3 Lys. If an ortholog has two or fewer residues changed, the changes are shown below the representative sequence. More-divergent termini within the orthologous group are shown in their entirety. Acidic and basic residues are shown in capital letters, and two or more consecutive charged residues are underlined. The H. somnus sequence comes from a cryptic prophage (29). A compilation of holin sequences can be found in Bläsi and Young (42) and in Young (41). The phage N15 holin sequence was obtained from R. Hendrix (19). Also shown are the C-terminal sequences of the predicted products of modified S alleles where a nucleotide sequence coding for an oligohistidine tag was inserted correctly (S $tau$ 94) and incorrectly (S $tau$ 94x, S $tau$ 94z) after codon 94 (35).

	MATERIALS AND METHODS

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Bacterial strains, bacteriophages, plasmids, and growth conditions. The Escherichia coli strains, bacteriophages, and plasmids used in this study are listed in Table 1. Standard bacterial brothmedia, plates, and top agar (Luria-Bertani [LB] and tryptone broth[TB]) were used (26). Unless indicated otherwise, bacterialcultures were grown in LB broth medium supplemented with ampicillin(Ap) (100 mg/ml; Sigma) to maintain selection of plasmids. Forsome plating assays, TB was also used as indicated. Growth andlysis were monitored by measuring the optical density at either550 or 600 nm, as indicated, by using a Gilford Stasar III sippingspectrophotometer.

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TABLE 1. Bacterial strains, plasmids, and phages used in this study

$lambda$ methods. Plating of phage $lambda$ was done by dilution with $lambda$ dil (5 mM MgSO₄, 0.01% gelatin, 10 mM Tris-HCl [pH 7.4]) and mixing 0.1 ml ofthe dilution with 0.1 ml of a fresh overnight of MC4100 (nonsuppressinglawn) or MS59 (suppressing lawn), grown either in TB or LB asindicated. This was followed by incubation at room temperaturefor 30 min and mixing with 3 ml of molten top LB or TB agar; themixtures were then poured onto fresh LB or TB plates. The plateswere incubated for at least 7 h at 37°C before they were scoredfor plaques. Lysogens were selected by infecting saturated mixturesthat had been incubated overnight with a lysate or plaque resuspendedin $lambda$ dil, streaking onto a LB-kanamycin (Km) plate, and incubationovernight at 30°C. The passive lysogeny assay was done as previouslydescribed (21). Briefly, lysates of non-plaque-forming bacteriophagecarrying a Km resistance marker are incubated with the lysogenMH760 $lambda$ for 1 h and then plated at various dilutions on LB-Km plates.Colonies arising after overnight incubation at 37°C are countedand compared with counts obtained with a known titer of a plaque-formingbacteriophage carrying the same drug resistancemarker.

Selection of plaque-forming pseudorevertant of SA52G mutant. A lysate of $lambda$ bj1, which carries the SA52G allele and has a severe defect in plaque formation (Table 1) (21), was platedon an MC4100 lawn. Small plaques were picked, purified by replating,and then picked again with a Pasteur pipet into $lambda$ dil. After vortexmixing with a drop of CHCl₃, the suspension was used to lysogenizeMC4100 on LB-Km as described previously (21). Individual lysogenswere purified and tested for lysis kinetics after thermal inductionas described previously (21).

Site-directed mutagenesis and cloning of the S mutant alleles. Amber (UAG) nonsense codons were individually introduced by replacing C-terminal codons specifying charged amino acids startingat codon position 92 (see Fig. 1). The mutant sequences were generatedby oligonucleotide site-directed mutagenesis according to themethod of Kunkel et al. (23) by using the single-stranded DNAtemplates M13SRRz and M13S105RRz prepared from the dut ung strainCJ236. For clarity, S⁺ alleles are defined as those in which the normal translationalstart is used (i.e., so that both S107 and S105 proteins are produced),whereas S105 and S107 refer to S alleles in which a CUG codonreplaces the start codon at position 1 and position 3, respectively,and thus only the indicated S gene product is produced. All oligonucleotidesused as mutagenic primers were complementary to the S coding sequence,except for the underlined mismatches. The mutations generatedare given in parentheses: 5'-GAAGCGCTAGATAAGC-3' (Lys92am), 5'-GCAGCGAACTATTTGATAA-3'(Arg93am), 5'-CTCCGGCTTTCTAAGCAGCG-3' (Lys97am), 5'-CTACTCCGGCCTATTTAGCAGC-3'(Lys98am), 5'-GATTTCTACCATCCTATACTCCGG-3' (Glu102am), and 5'-GATTTCTACCCTATTCTACTC-3'(Asp103am).

The $lambda$ S105RRz cassette was reisolated on an EcoRI/HindIII fragment from M13S105RRz DNA and cloned into the corresponding sitesdownstream of the lacPO promoter-operator region in pBH20, whichresulted in plasmid pPF110. After the mutations were verifiedby sequencing, the respective S alleles were isolated togetherwith the accessory lysis genes R and Rz on an EcoRI/HindIII fragmentand cloned into the EcoRI/HindIII restriction sites of the cloningector pBH20 (Table 1). Plasmids pPF101 and pPF102 carry the ambermutations at positions K92 and R93, respectively, in S. Cloningof the mutant S105 alleles into vector pBH20 resulted in plasmidspPF113 (K97am), pPF114 (K98am), pPF115 (E102am), and pPF116 (D103am).Transfer of the K92am, K97am, E102am, and D103am mutant allelesto $lambda$ by recombination and the determinations of the burst sizewere done out as previously described (31).

Determination of membrane topology. E. coli MC4100(pBS112), carrying the S107 allele (5) was grown in M9 maltose medium for $lambda$ CE6 infection as described previously(9), except that rifampin (100 µg/ml) was added at 15 min afterinfection. A 10-ml volume of culture was pulse-labelled with 200µCi of [³⁵S]methionine (>1,000 Ci/mmol; NEN) for 5 min, beginning at 25min after infection. Preparation of inverted membrane vesicles(IMV) and spheroplasts and the proteinase K digestions were doneas described elsewhere (15, 22, 27), with the followingmodifications. For spheroplast samples, 4 ml of labelled culturewas divided into 1-ml aliquots and placed in four microfuge tubes.After the cells were pelleted by centrifugation for 1 min, thepellet was resuspended in 100 µl of spheroplasting buffer (40%sucrose, 20 mM EDTA, 60 mM Tris-HCl [pH 8]) and treated with lysozyme(10 µg/ml; Sigma) at 37°C. One sample was treated with 2% TritonX-100 to lyse the cells prior to proteinase K treatment. ProteinaseK digestion was halted with 2 mM phenylmethylsulfonyl fluoride(Sigma). After proteinase K treatment, spheroplasts were collectedby pelleting in a microfuge and then resuspended in 25 µl of 1%sodium dodecyl sulfate (SDS)-1 mM EDTA for 40 s before dilutionto a final volume of 500 µl with TSET (150 mM NaCl, 1 mM EDTA,2% Triton X-100, 50 mM Tris-HCl [pH 8.0]) for immunoprecipitation.For IMV samples, the remaining 6 ml of labelled culture was pelletedas described above and resuspended in 1 ml of French press buffer(20 mM EDTA, 60 mM Tris-HCl [pH 8]). The suspension was disruptedby passage through a French pressure cell (SLM-Aminco) at 16,000lb/in², generating the IMV sample, which was freed of unlysed cellsby centrifugation in a microfuge tube at 3,000 × g for 1 min.The resulting IMV sample was divided into aliquots and placedin 6 microfuge tubes and then treated with proteinase K as describedabove for different time intervals. One sample was lysed withdetergent prior to digestion, as described above. After the digestionwas stopped with 2 mM phenylmethylsulfonyl fluoride, the IMV wereharvested by centrifugation at 100,000 × g as described earlier(22). The cytoplasmic membrane protein fraction was obtainedby resuspending the membrane pellet in 200 µl of membrane extractionbuffer (10 mM Tris-HCl [pH 8], 35 mM MgCl₂, 1% Triton X-100),extraction with stirring for 1 h, and removal of the insolubledebris by recentrifugation at 100,000 × g. The extract (ca. 50µl) was diluted with 450 µl of TSET buffer forimmunoprecipitation.

Immunoprecipitation was carried out with antibody raised against a synthetic peptide corresponding to the C-terminal 16 residuesof S, as described previously (10). In vitro translation ofS mRNA and autoradiography was performed as described previously(9).

	RESULTS

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C-terminal domain of the $lambda$ holin is disposed in the cytoplasm. As a first step in determining the membrane topology of the S holin, the localization of the C-terminal domain was investigatedby protease accessibility analysis in inverted membrane vesiclesand in spheroplasts. To maximize labelling of the S protein andto reduce the background, the labelling was done with cells carryingplasmids in which the S reading frame is transcribed from a T7RNA polymerase promoter and fused to the efficient ribosome bindingsite of T7 gene 10. S protein has been shown to accumulate ina fully functional form in the cytoplasmic membrane under theseconditions (34). Initial experiments were done with the S107allele because expression of the S⁺ allele is incompatible with efficient spheroplasting (32).The results show that the C-terminal domain of the S107 proteinis susceptible to exogenous protease in inverted membrane vesiclesbut not in spheroplasts (Fig. 3). The faint protease-resistantband presumably corresponds to the small fraction of inner membranevesicles which are not inverted. Although spheroplasts could notbe reproducibly prepared, similar results were obtained with proteasetreatment of inner membrane vesicles using the S⁺ allele (not shown). The simplest interpretation is that, as expectedfrom sequence analysis of the S gene, the highly charged C-terminaldomain is cytoplasmic. Although in any model for S topology atleast one loop between transmembrane domains should be accessiblefrom the periplasmic face, the fact that the S protein is completelyprotected in spheroplasts indicates that the loop is not sufficientlyexposed to be accessible to the protease. (The accessibility ofthe periplasmic face of the spheroplasts prepared by this techniquewas verified by determining the proteolysis products of labelledTsr protein [not shown]).

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FIG. 3. The C-terminal domain of the S protein is accessible to proteases in inverted membrane vesicles. E. coli MC4100(pBS112) cells were infected with $lambda$ CE6 and labelled with [³⁵S]methionine at 25 min after infection. Spheroplasts and IMV, treated with proteinase K, with or without detergent, for various times as indicated. Each sample was subjected to immunoprecipitation with anti-S antibody (9), and the immunoprecipitate was analyzed by SDS-polyacrylamide gel electrophoresis and autoradiography. Lanes: 1, in vitro translation products of S⁺ mRNA, as described previously (9); 2 to 5, spheroplast samples; 6 to 11, IMV samples.

Effect of C-terminal amber mutations on lysis and its timing. To test the hypothesis that some or all of the C-terminal domain might be dispensable for lysis, nonsense mutations in a numberof distal codons of the S gene were created by site-directed mutagenesis.The different S alleles were cloned as SRRz lysis gene "cassettes"under lacPO control on a moderate-copy-number plasmid, resultingin the pPF series of plasmids (Table 1). Remarkably, all of theS amber mutant alleles truncated at codon 93 or beyond were lysisproficient, confirming that most of the C-terminal domain of Sis unnecessary for "hole formation" (Table 2). In addition, allof the lysis-proficient alleles shared with the parental allelethe property of premature triggering by the addition of an energypoison, indicating that the intrinsic components of lysis timingwere retained in these mutants. However, induction of the K92amallele does not result in lysis. Addition of chloroform, whichpermeabilizes the inner membrane, results in the immediate lossof turbidity, which shows that the lysis defect is not due toa deficiency in endolysin activity (not shown). We conclude thatthe K92am is an absolute-lysis-defective allele. The K92am alleleis recessive, as determined by its lack of an effect on lysiskinetics when expressed in trans to the S⁺ allele borne on a compatible plasmid (not shown). It is unclearwhether the defect is due to the inability of the mutant proteinto accumulate in the membrane, because the available anti-S antibodywas raised against an oligopeptide corresponding to the C-terminalsequence, which prevents detection of any of the C-terminal ambermutants in immunoblots (13). Nevertheless, the recessive characterof the K92am lysis defect is consistent with the idea that atleast one positively charged residue at the C-terminal end isrequired for insertion in the membrane or the attainment of propertopology.

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TABLE 2. Lysis phenotypes of C-terminal S mutants

As detailed above, the N terminus of the S107 gene product of S determines its inhibitor function. We wanted to test if theC terminus, although largely dispensable for lysis, was also requiredfor the ability of S107 to modulate lysis time. When the S alleleswere expressed from a moderate-copy-number plasmid in trans toan S107 allele (which produces only the S107 product) on a compatibleplasmid, the lysis times for all of the C-terminal truncationswere normally retarded, relative to the retardation seen for full-lengthS (Table 3). Thus, the C-terminal domain does not seem to berequired for intermolecular interactions, at least not for thoseinvolved in the inhibitor function.

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TABLE 3. Effect of endolysin or S107 inhibitor supplied in trans

For the truncations at codon 93 or beyond, there is a general correlation between the length of the residual C-terminal domainand the timing of lysis (Table 2). The two shortest truncationswhich were lysis proficient both lysed earlier than the wild-typeallele (Table 2). However, in two cases, the D103am and E102am,the onset of lysis was followed by a very gradual loss of turbidity.Moreover, even the addition of CHCl₃ did not accelerate lysisdramatically, indicating a reduced level of R expression (notshown). It seemed likely that the placement of the nonsense codonsin these alleles were disrupting translation of the R gene andthus disturbing the stability of the polycistronic mRNA producedfrom the cloned lysis gene cassette in the lacPO plasmid vector.Inspection of the sequence shows that the D103am mutation eliminatesthe normal start codon of R, and thus the residual bacteriolyticactivity must come from downstream translational start sites (Fig.4). The E102am mutation does not directly affect the Shine-Dalgarnosequence or the start codon, but the intervening nucleotide sequenceis altered. Thus, the lack of endolysin activity here, too, islikely to be due to a translational defect. In both cases, supplyingthe R gene product in trans from a compatible plasmid resultedin more-saltatory lysis profiles, although the timing of lysisonset was not altered (Table 3).

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FIG. 4. Sequence of S-R intergenic region. The sequence of the S-R intergenic region is shown, with the corresponding C-terminal sequences of S and N-terminal sequences of R. Also shown are the sequences of the D103am and E102am mutants. In each case, the presumptive Shine-Dalgarno sequence for R is underlined and both the wild-type start codon and the first downstream alternative start codon for R are shown in boldface. Asterisks denote the sequence alterations resulting from the creation of the corresponding amber codons in the S reading frame.

Characterization of $lambda$ Sam recombinants. To achieve a more robust expression system, the nonsense alleles were recombined into the normal phage context, where S isunder its cognate transcriptional controls and where the Q-mediatedtranscription is much less susceptible to polarity effects (12).The standard $lambda$ vector used for recombining the plasmid S allelesis $lambda$ kan, which carries deletions of three nonessential regionsof the phage, a Tn903 insertion to provide Km^r for selecting lysogens and a deletion of the S and R genes (31).Recombination with the plasmids results in transfer of the S andR alleles to the phage context. Thermal induction of the lysogenby brief aeration at 42°C allows synchronous initiation of thephage vegetative cycle throughout the culture and thus allowsrather precise assessment of the lysis kinetics associated witheach S allele by monitoring the A₅₅₀ during growth under standardconditions (21, 31). Moreover, plating efficiency and plaquesize could be assessed as measures of the biological functionof the S allele. Figure 5 shows a representative induction experimentwhich shows that the K92am allele is lysis defective in the phagecontext. In addition, lysis can be accomplished in the inducedK92am lysogen by adding CHCl₃ but not cyanide, indicating thatthe defect is due to an absence of functional S protein and notto the production of endolysin (not shown). Three other truncationalleles are lysis proficient, although the lysis profile of D103amis significantly more gradual, distinctly different from the sharplydefined, saltatory lysis profiles exhibited by the parental andK97am alleles. The E102 allele exhibited variable lysis kinetics,although it was always triggered somewhat earlier than the parentalallele (Fig. 5). In addition, the K97am allele, which had theshortest lysis-proficient C-terminal domain of the alleles crossedinto the phage context, exhibited onset of lysis much earlierthan the parental allele. The plating characteristics of theseS mutants were also different. As expected, PFU were detectedin the lysate from the nonlysing alleles at a level consistentwith spontaneous reversion (Table 4). PFU were produced at aboutequal efficiency for the parental and E102am alleles, and at aslightly reduced level, with significantly smaller plaque size,for the D103am allele. In contrast, the early lysis allele K97amexhibited a pronounced plating defect, with reduced numbers ofpinpoint plaques under optimal plating conditions and with noplaques under more-stringent conditions (Table 4). On a suppressorlawn, all of the mutant lysates generated normal numbers of plaques.To determine plating efficiency, the number of Km^r transducing particles was assessed by a passive recombinationassay, where cells with a resident prophage are infected witheach lysate and plated on antibiotic medium. This assay revealedthat the burst size in the K97am allele was reduced to about 20%that of the parental allele, presumably because the early onsetof lysis aborts the vegetative phase before its most productiveperiod.

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FIG. 5. Lysis profiles for induced lysogens with C-terminal alterations in S. (A) Lysogens of $lambda$ b515 b519 Tn903 cI857 nin5 S105 carrying S alleles with different C-terminal amber mutations were thermally induced in logarithmic phase and monitored for lysis by measuring the A₅₅₀. Representative lysis profiles are shown for all alleles, including two profiles showing the variability of the K97am lysis kinetics. Symbols:

, parental (no truncation);

, D103am; $black-lozenge$ , E102am; $down-triangle$ and $black-down-triangle$ , K97am; ×, K92am. (B) Lysogens of $lambda$ kan (

) and the isogenic phages $lambda$ bj1 (SA52G [

]) and $lambda$ aj1 (plaque-forming revertant of $lambda$ bj1 [ $diamond$ ]) were thermally induced and monitored as in panel A.

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TABLE 4. Plating phenotypes of $lambda$ Sam recombinants

C-terminal frameshift mutation suppresses a severe early lysis defect. A similar but more extreme plating defect was found for the allele A52G due to a more exacerbated early lysis time, 19 minafter induction, before the first progeny virion has been assembledintracellularly in the average induced cell (21). This mutanthas an absolute plating defect under stringent plating conditions.Pseudorevertants were isolated as small plaque-formers under theseconditions and were shown to have regained an extended vegetativeperiod (Fig. 5B). Sequence analysis of a pseudorevertant, $lambda$ aj1,revealed that the suppressing mutation was a frameshift withinthe 97th codon of S. The new reading frame specifies a C-terminalsequence which, although shorter and completely unrelated to theoriginal S sequence, has a predicted net increase of four positivecharges (Fig. 1). Thus, a C-terminal change resulting in a changein the electrostatic charge of the C terminus, without conservationof sequence, can compensate for an alteration in the intrinsictiming of the holin. Consistent with this finding, other S distalframeshifts, created by errors in the process of inserting oligohistidinetags into sites in the C-terminal domain (35), were found toretain normal lysis timing. In these two alleles, the nonhomologoussequence begins after position 94 and generates C-terminal sequencesunrelated to the parental allele but with net predicted chargessimilar to that of the parental allele (Fig. 2). In both cases,the S alleles are fully functional, with similar or even acceleratedlysis kinetics (35). We conclude that the sequence of the C-terminaldomain does not serve a specific functional role in the abilityof S to mediate hole formation but instead serves as a reservoirof charge which serves to regulate the timing oflysis.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Implications for holin topology. We have demonstrated that the C-terminal domain of S is located in the cytoplasm. While this result is not unexpected sinceits sequence is so rich in acidic and basic residues, it doesreduce the number of reasonable models for the transmembrane topologyof S. As noted above, the S sequence has three putative transmembranedomains, although the putative TM3 domain is rather rich in hydroxylatedresidues and is not recognized by available computer algorithmsas likely to be membrane embedded (40). Requiring the C-terminaldomain to be cytoplasmically disposed results in opposite locationsfor the N terminus, depending on whether two or three transmembranedomains are present (Fig. 6, center and right models). The mostsuccessful primary sequence tool for predicting membrane topologyis defined by the von Heijne rules, which state that the cytoplasmicdisposition of positively charged residues immediately flankingeach transmembrane domain will be maximized (14, 39). By thiscriterion, a model with three transmembrane domains is favored(Fig. 6, right), not only for S but also for the other nonorthologousclass I holins identified in phages of gram-negative hosts (P1LydA, P2 Y, N15 holin, and PRD1 OrfM). However, there are numerousclass II holins which have shorter primary sequences which, byinspection, clearly can have only have two transmembrane domains(42). These holins, at least one of which has already been shownto complement $lambda$ S efficiently (7), also have highly chargedC-terminal domains, which presumably are also located in the cytoplasm(Fig. 2 and 6). The membrane topology of class I holins has beenelusive (6). If all three potential transmembrane domains arein the bilayer and since the C terminus was found to be in thecytoplasm, then the N terminus should be on the periplasmic sideof the membrane. Chemical modification studies of S in isolatedmembrane vesicles support the existence of the third transmembranedomain (18). Moreover, recent experiments have shown that asecretory signal sequence fused to the N terminus of S facilitatesS hole formation in a signal peptidase-dependent manner, stronglysupporting the notion that S function requires its N terminusof S to cross the membrane at some point (17). Thus, accordingto this view, the positive charge on the N terminus, which confersinhibitor function on S107, does so by retarding this translocation(6). Interestingly, the dual-start motif also functions asa regulatory feature in the class II holins, where translocationof the N terminus to the periplasm is, by inspection, highly unlikely(1).

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FIG. 6. Possible membrane topologies of S. Depicted are putative membrane topologies for prototype class II (S from phage 21; left) and class I (S from phage $lambda$ ; middle and right) holin proteins. The inner membrane is shown as shaded area with positively charged periplasmic and negatively charged cytoplasmic surfaces. Transmembrane helical domains are represented as white rectangles spanning the membrane. Basic residues in putative solvent-exposed domains are shown for both 21 and $lambda$ holins.

Regulatory, but not functional role, for the C terminus. In addition, we have shown that most of the C-terminal charged domain of S is not required for the ability to form the innermembrane lesions ("holes") necessary for the R endolysin to gainaccess to the cell wall and effect lysis. Only one positivelycharged residue, at codon 92, is required for lytic function.The positively charged residue may be required for the abilityof S to integrate in the membrane or, as demonstrated for derivativesof the Lep protein, to define the orientation of the adjacenttransmembrane domain (14). Moreover, the timing of lysis isloosely correlated with the number of positively charged residuesor the total net positive charge in the C terminus. This conclusionstems from the lysis kinetics exhibited by the C-terminal ambermutants. Additional evidence is provided by the fact that theframeshift mutation isolated as an intragenic suppressor of anearly lysis mutation has a scrambled sequence beyond codon 97.In the frameshift mutant which suppresses A52G, the C-terminalnine residues, containing one basic and two acidic residues, arereplaced with a different six-residue sequence containing threebasic residues. Apparently, this change of +4 positive chargesacts to retard the intrinsic tendency of the A52G mutation totrigger hole formation early. Similar frameshifts were fortuitouslyfound during oligohistidine tag mutagenesis of the S sequence(35). The insertion frameshifts also scramble the C-terminalsequence but result in predicted charges of either +3 or +4, andthe lysis onset is either as fast or even faster than with theparental S. Moreover, in a selection for S genes with reducedlethality, Raab et al. (30, 31) isolated an S missense mutant,E102K, a change which increases the net positive charge of theC-terminal domain by two and results in a 19-min delay in lysisonset. Interestingly, the E102K allele is recessive, indicatingthat the timing delay associated with the C-terminal charged domainis a cis effect. Thus, the primary function of the C-terminaldomain appears not to be as a structural element in the lethal"hole" but instead in the proper scheduling of the hole-formingevent, with an increasing positive charge being directly correlatedto a slowing of the onset of lysis. This does not imply that theC-terminal domain is unnecessary for the biological function ofthe S protein. It should be noted that the K97am allele is alsoformally a Sam defective allele, like the Sam7 null allele (16),despite the fact that it supports complete lysis of the host.This illustrates that the timing and hole-forming functions ofthe S gene are both essential to $lambda$ .

Lytic function defined by the hydrophobic core. A similar regulatory role has been suggested for the N-terminal sequence that precedes the first transmembrane domain (6,36). To a significant extent, the lysis "clock" is set by therelative proportion of S105 and S107 products. In effect, thisproportion specifies the average charge on the N-terminal sidechains of the population of S molecules in the membrane, and thedelay in lysis needed for accumulation of progeny virions appearsto be a direct function of the positive charge on the N terminus(4, 28). Moreover, as an adventitious result of PCR-mediatedsite-directed mutagenesis, mutants have been isolated with additionalbasic residues in the first 10 positions, and these alleles exhibitnegative-dominant lysis delay phenotypes (35). This suggeststhat the N-terminal domain primarily acts to regulate lysis timing,again with an increasing positive charge being correlated withthe retardation of lysis onset. Thus, both N- and C-terminal domainsappear to function primarily as inhibitory domains which primarilyregulate by electrostatic means. In other words, the intrinsichole-forming capacity of the S protein appears to be specifiedby its hydrophobic core (6). This in turn suggests that theprotein-protein interactions which determine the specificity ofthe oligomeric hole structure are probably within the membrane-embeddedsequences. This notion is consistent with the fact that the S107inhibitor can still exert its inhibitory function on the productsof the C-terminal truncations (see Table 3). Moreover, the greatpreponderance of missense mutations which inactivate the lethalcapacity of S cluster in the first two transmembrane domains (30,31). The fact that many of these mutations are relatively subtleand do not reduce the hydrophobic character (i.e., A48V, M50I,A52V, and L25F) suggests that an intimate interaction betweentransmembrane domains is essential for hole formation. Similarconclusions have been given a biochemical and structural basisby Engelman and coworkers, who have shown that altering the bulkof residues in the transmembrane domain of glycophorin can abolishthe ability of that transmembrane domain to form dimers (24).Biochemical analysis of S may be accelerated by the finding thatboth N- and C-terminal extrema are unnecessary for holeformation.

	ACKNOWLEDGMENTS

We thank other members of the two laboratories for their help and constructive criticism. Amanda Jochen is specifically acknowledgedfor isolating the aj1 pseudorevertant. We also appreciate, asalways, the patient clerical services of SharyllPressley.

Work in the Young laboratory is supported by funding from project Public Health Service grant GM27099 and by funds from theCollege of Agriculture, Texas A&M University, and the Texas AgriculturalExperiment Station. Work in the Bläsi laboratory is supportedby grant P12220MOB from the Austrian Science Foundation and grant6170 from the Austrian NationalBank.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry and Biophysics, Texas A&M University, College Station, TX77843-2128. Phone: (409) 845-2087. Fax: (409) 862-4718. E-mail:ryland{at}tamu.edu.

Present address: Department of Microbiology, University of Texas, ESB 226, Austin, TX 78712-1095.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Barenboim, M., C.-Y. Chang, F. dib Hajj, and R. Young. A holin and its inhibitor are both encoded by the phage 21 S gene. Mol. Microbiol., in press.

2. Bienkowska-Szewczyk, K., B. Lipinska, and A. Taylor. 1981. The R gene product of bacteriophage $lambda$ is the murein transglycosylase. Mol. Gen. Genet. 184:111-114[Medline].

3. Bläsi, U., C.-Y. Chang, and R. Young. Unpublished data.

4. Bläsi, U., C.-Y. Chang, M. T. Zagotta, K. Nam, and R. Young. 1990. The lethal $lambda$ S gene encodes its own inhibitor. EMBO J. 9:981-989[Medline].

5. Bläsi, U., K. Nam, D. Hartz, L. Gold, and R. Young. 1989. Dual translational initiation sites control function of the $lambda$ S gene. EMBO J. 8:3501-3510[Medline].

6. Bläsi, U., and R. Young. 1996. Two beginnings for a single purpose: the dual-start holins in the regulation of phage lysis. Mol. Microbiol. 21:675-682[Medline].

7. Bonovich, M. T., and R. Young. 1991. Dual start motif in two lambdoid S genes unrelated to $lambda$ S. J. Bacteriol. 173:2897-2905[Abstract/Free Full Text].

8. Casjens, S. R., K. Eppler, R. Parr, and A. R. Poteete. 1989. Nucleotide sequence of the bacteriophage P22 gene 19 to 3 region: identification of a new gene required for lysis. Virology 171:588-598[Medline].

9. Chang, C.-Y., K. Nam, U. Bläsi, and R. Young. 1993. Synthesis of two bacteriophage $lambda$ S proteins in an in vivo system. Gene 133:9-16[Medline].

10. Chang, C.-Y., K. Nam, and R. Young. 1995. S gene expression and the timing of lysis by bacteriophage $lambda$ . J. Bacteriol. 177:3283-3294[Abstract/Free Full Text].

11. Cheng, X., X. Zhang, J. W. Pflugrath, and F. W. Studier. 1994. The structure of bacteriophage T7 lysozyme, a zinc amidase and an inhibitor of T7 RNA polymerase. Proc. Natl. Acad. Sci. USA 91:4034-4038[Abstract/Free Full Text].

12. Forbes, D., and I. Herskowitz. 1982. Polarity suppression by the Q gene product of phage lambda. J. Mol. Biol. 160:549-569[Medline].

13. Fraisl, P., and R. Young. Unpublished data.

14. Gafvelin, G., and G. von Heijne. 1994. Topological "frustration" in multispanning E. coli inner membrane proteins. Cell 77:401-412[Medline].

15. Geller, B. L. 1990. Electrochemical potential releases a membrane-bound secretion intermediate of maltose-binding protein in Escherichia coli. J. Bacteriol. 172:4870-4876[Abstract/Free Full Text].

16. Goldberg, A. R., and M. Howe. 1969. New mutations in the S cistron of bacteriophage lambda affecting host cell lysis. Virology 38:200-202[Medline].

17. Graschopf, A., and U. Bläsi. Molecular function of the dual-start motif in the lambda S holin. Submitted for publication.

18. Gründling, A., and R. Young. Unpublished data.

19. Hendrix, R. 1992. Personal communication.

20. Itakura, K., T. Hirose, R. Crea, A. Riggs, H. L. Heyneker, F. Boliver, and H. W. Boyer. 1979. Expression in Escherichia coli of a chemically synthesized gene for the hormone somatostatin. Science 198:1056-1063.

21. Johnson-Boaz, R., C.-Y. Chang, and R. Young. 1994. A dominant mutation in the bacteriophage lambda S gene causes premature lysis and an absolute defective plating phenotype. Mol. Microbiol. 13:495-504[Medline].

22. Kuhn, A., H.-Y. Zhu, and R. E. Dalbey. 1990. Efficient translocation of positively charged residues of M13 procoat protein across the membrane excludes electrophoresis as the primary force for membrane insertion. EMBO J. 9:2385-2389[Medline].

23. Kunkel, T. A., J. D. Roberts, and R. A. Zakour. 1987. Rapid and efficient site specific mutagenesis without phenotypic selection. Methods Enzymol. 154:367-382[Medline].

24. Lemmon, M. A., J. M. Flanagan, H. R. Treutlein, J. Zhang, and D. M. Engelman. 1992. Sequence specificity in the dimerization of transmembrane alpha-helices. Biochemistry 31:12719-12725[Medline].

25. Messing, J., R. Crea, and P. H. Seeburg. 1981. A system for shotgun DNA sequencing. Nucleic Acids Res. 9:309-321[Abstract/Free Full Text].

26. Miller, J. H. 1992. A short course in bacterial genetics: a laboratory manual and handbook for Escherichia coli and related bacteria. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

27. Müller, M., and G. Blobel. 1984. In vitro translocation of bacterial proteins across the plasma membrane of Escherichia coli. Proc. Natl. Acad. Sci. USA 81:7421-7425[Abstract/Free Full Text].

28. Nam, K., U. Bläsi, M. T. Zagotta, and R. Young. 1990. Conservation of a dual-start motif in P22 lysis gene regulation. J. Bacteriol. 72:204-211.

29. Pontarollo, R. A., C. R. Rioux, and A. A. Potter. 1997. Cloning and characterization of bacteriophage-like DNA from Haemophilus somnus homologous to phages P2 and HP1. J. Bacteriol. 179:1872-1879[Abstract/Free Full Text].

30. Raab, R., G. Neal, J. Garrett, R. Grimaila, R. Fusselman, and R. Young. 1986. Mutational analysis of bacteriophage lambda lysis gene S. J. Bacteriol. 167:1035-1042[Abstract/Free Full Text].

31. Raab, R., G. Neal, C. Sohaskey, J. Smith, and R. Young. 1988. Dominance in lambda S mutations and evidence for translational control. J. Mol. Biol. 199:95-105[Medline].

32. Reader, R. W., and L. Siminovitch. 1971. Lysis defective mutants of bacteriophage lambda: on the role of the S function in lysis. Virology 43:623-637[Medline].

33. Silhavy, T. J., M. L. Berman, and L. W. Enquist. 1984. Experiments with gene fusions. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

34. Smith, D. L., D. K. Struck, J. M. Scholtz, and R. Young. 1998. Purification and biochemical characterization of the lambda holin. J. Bacteriol. 180:2531-2540[Abstract/Free Full Text].

35. Smith, D. L., and R. Young. 1998. Oligohistidine tag mutagenesis of the $lambda$ holin gene. J. Bacteriol. 180:4199-4211[Abstract/Free Full Text].

36. Steiner, M., and U. Bläsi. 1993. Charged amino-terminal amino acids affect the lethal capacity of lambda lysis proteins S107 and S105. Mol. Microbiol. 8:525-533[Medline].

37. Studier, F. W., and B. A. Moffatt. 1986. Use of bacteriophage T7 RNA polymerase to direct selective high-level expression of cloned genes. J. Mol. Biol. 189:113-130[Medline].

38. Tedin, K., A. Resch, M. Steiner, and U. Bläsi. 1995. Dual translational start motif evolutionarily conserved in the holin gene of Bacillus subtilis phage $phi$ 29. Virology 206:479-484[Medline].

39. von Heijne, G. 1989. Control of topology and mode of assembly of a polytopic membrane protein by positively charged residues. Nature 341:456-458[Medline].

40. Young, R. Unpublished data.

41. Young, R. 1992. Bacteriophage lysis: mechanism and regulation. Microbiol. Rev. 56:430-481[Abstract/Free Full Text].

42. Young, R., and U. Bläsi. 1995. Holins: form and function in bacteriophage lysis. FEMS Microbiol. Rev. 17:191-205[Medline].

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	ALL ASM JOURNALS

1.	Barenboim, M., C.-Y. Chang, F. dib Hajj, and R. Young. A holin and its inhibitor are both encoded by the phage 21 S gene. Mol. Microbiol., in press.
2.	Bienkowska-Szewczyk, K., B. Lipinska, and A. Taylor. 1981. The R gene product of bacteriophage $lambda$ is the murein transglycosylase. Mol. Gen. Genet. 184:111-114[Medline].
3.	Bläsi, U., C.-Y. Chang, and R. Young. Unpublished data.
4.	Bläsi, U., C.-Y. Chang, M. T. Zagotta, K. Nam, and R. Young. 1990. The lethal $lambda$ S gene encodes its own inhibitor. EMBO J. 9:981-989[Medline].
5.	Bläsi, U., K. Nam, D. Hartz, L. Gold, and R. Young. 1989. Dual translational initiation sites control function of the $lambda$ S gene. EMBO J. 8:3501-3510[Medline].
6.	Bläsi, U., and R. Young. 1996. Two beginnings for a single purpose: the dual-start holins in the regulation of phage lysis. Mol. Microbiol. 21:675-682[Medline].
7.	Bonovich, M. T., and R. Young. 1991. Dual start motif in two lambdoid S genes unrelated to $lambda$ S. J. Bacteriol. 173:2897-2905[Abstract/Free Full Text].
8.	Casjens, S. R., K. Eppler, R. Parr, and A. R. Poteete. 1989. Nucleotide sequence of the bacteriophage P22 gene 19 to 3 region: identification of a new gene required for lysis. Virology 171:588-598[Medline].
9.	Chang, C.-Y., K. Nam, U. Bläsi, and R. Young. 1993. Synthesis of two bacteriophage $lambda$ S proteins in an in vivo system. Gene 133:9-16[Medline].
10.	Chang, C.-Y., K. Nam, and R. Young. 1995. S gene expression and the timing of lysis by bacteriophage $lambda$ . J. Bacteriol. 177:3283-3294[Abstract/Free Full Text].
11.	Cheng, X., X. Zhang, J. W. Pflugrath, and F. W. Studier. 1994. The structure of bacteriophage T7 lysozyme, a zinc amidase and an inhibitor of T7 RNA polymerase. Proc. Natl. Acad. Sci. USA 91:4034-4038[Abstract/Free Full Text].
12.	Forbes, D., and I. Herskowitz. 1982. Polarity suppression by the Q gene product of phage lambda. J. Mol. Biol. 160:549-569[Medline].
13.	Fraisl, P., and R. Young. Unpublished data.
14.	Gafvelin, G., and G. von Heijne. 1994. Topological "frustration" in multispanning E. coli inner membrane proteins. Cell 77:401-412[Medline].
15.	Geller, B. L. 1990. Electrochemical potential releases a membrane-bound secretion intermediate of maltose-binding protein in Escherichia coli. J. Bacteriol. 172:4870-4876[Abstract/Free Full Text].
16.	Goldberg, A. R., and M. Howe. 1969. New mutations in the S cistron of bacteriophage lambda affecting host cell lysis. Virology 38:200-202[Medline].
17.	Graschopf, A., and U. Bläsi. Molecular function of the dual-start motif in the lambda S holin. Submitted for publication.
18.	Gründling, A., and R. Young. Unpublished data.
19.	Hendrix, R. 1992. Personal communication.
20.	Itakura, K., T. Hirose, R. Crea, A. Riggs, H. L. Heyneker, F. Boliver, and H. W. Boyer. 1979. Expression in Escherichia coli of a chemically synthesized gene for the hormone somatostatin. Science 198:1056-1063.
21.	Johnson-Boaz, R., C.-Y. Chang, and R. Young. 1994. A dominant mutation in the bacteriophage lambda S gene causes premature lysis and an absolute defective plating phenotype. Mol. Microbiol. 13:495-504[Medline].
22.	Kuhn, A., H.-Y. Zhu, and R. E. Dalbey. 1990. Efficient translocation of positively charged residues of M13 procoat protein across the membrane excludes electrophoresis as the primary force for membrane insertion. EMBO J. 9:2385-2389[Medline].
23.	Kunkel, T. A., J. D. Roberts, and R. A. Zakour. 1987. Rapid and efficient site specific mutagenesis without phenotypic selection. Methods Enzymol. 154:367-382[Medline].
24.	Lemmon, M. A., J. M. Flanagan, H. R. Treutlein, J. Zhang, and D. M. Engelman. 1992. Sequence specificity in the dimerization of transmembrane alpha-helices. Biochemistry 31:12719-12725[Medline].
25.	Messing, J., R. Crea, and P. H. Seeburg. 1981. A system for shotgun DNA sequencing. Nucleic Acids Res. 9:309-321[Abstract/Free Full Text].
26.	Miller, J. H. 1992. A short course in bacterial genetics: a laboratory manual and handbook for Escherichia coli and related bacteria. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
27.	Müller, M., and G. Blobel. 1984. In vitro translocation of bacterial proteins across the plasma membrane of Escherichia coli. Proc. Natl. Acad. Sci. USA 81:7421-7425[Abstract/Free Full Text].
28.	Nam, K., U. Bläsi, M. T. Zagotta, and R. Young. 1990. Conservation of a dual-start motif in P22 lysis gene regulation. J. Bacteriol. 72:204-211.
29.	Pontarollo, R. A., C. R. Rioux, and A. A. Potter. 1997. Cloning and characterization of bacteriophage-like DNA from Haemophilus somnus homologous to phages P2 and HP1. J. Bacteriol. 179:1872-1879[Abstract/Free Full Text].
30.	Raab, R., G. Neal, J. Garrett, R. Grimaila, R. Fusselman, and R. Young. 1986. Mutational analysis of bacteriophage lambda lysis gene S. J. Bacteriol. 167:1035-1042[Abstract/Free Full Text].
31.	Raab, R., G. Neal, C. Sohaskey, J. Smith, and R. Young. 1988. Dominance in lambda S mutations and evidence for translational control. J. Mol. Biol. 199:95-105[Medline].
32.	Reader, R. W., and L. Siminovitch. 1971. Lysis defective mutants of bacteriophage lambda: on the role of the S function in lysis. Virology 43:623-637[Medline].
33.	Silhavy, T. J., M. L. Berman, and L. W. Enquist. 1984. Experiments with gene fusions. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
34.	Smith, D. L., D. K. Struck, J. M. Scholtz, and R. Young. 1998. Purification and biochemical characterization of the lambda holin. J. Bacteriol. 180:2531-2540[Abstract/Free Full Text].
35.	Smith, D. L., and R. Young. 1998. Oligohistidine tag mutagenesis of the $lambda$ holin gene. J. Bacteriol. 180:4199-4211[Abstract/Free Full Text].
36.	Steiner, M., and U. Bläsi. 1993. Charged amino-terminal amino acids affect the lethal capacity of lambda lysis proteins S107 and S105. Mol. Microbiol. 8:525-533[Medline].
37.	Studier, F. W., and B. A. Moffatt. 1986. Use of bacteriophage T7 RNA polymerase to direct selective high-level expression of cloned genes. J. Mol. Biol. 189:113-130[Medline].
38.	Tedin, K., A. Resch, M. Steiner, and U. Bläsi. 1995. Dual translational start motif evolutionarily conserved in the holin gene of Bacillus subtilis phage $phi$ 29. Virology 206:479-484[Medline].
39.	von Heijne, G. 1989. Control of topology and mode of assembly of a polytopic membrane protein by positively charged residues. Nature 341:456-458[Medline].
40.	Young, R. Unpublished data.
41.	Young, R. 1992. Bacteriophage lysis: mechanism and regulation. Microbiol. Rev. 56:430-481[Abstract/Free Full Text].
42.	Young, R., and U. Bläsi. 1995. Holins: form and function in bacteriophage lysis. FEMS Microbiol. Rev. 17:191-205[Medline].

The C-Terminal Sequence of the Holin Constitutes a Cytoplasmic Regulatory Domain

The C-Terminal Sequence of the $lambda$ Holin Constitutes a Cytoplasmic Regulatory Domain