Your search keyword '"Host cell envelope"' showing total 12 results

1. The Mycobacteriophage Ms6 LysB

Author

José Moniz-Pereira, Adriano M Gigante, Paula Leandro, Francisco Olivença, Maria João Catalão, Madalena Pimentel, Sergio R. Filipe, DCV - Departamento de Ciências da Vida, UCIBIO - Applied Molecular Biosciences Unit, and Instituto de Tecnologia Química e Biológica António Xavier (ITQB)

Subjects

peptidoglycan binding, mycobacteria, Lysin, Peptidoglycan binding, Bacillus subtilis, Peptidoglycan, Microbiology, Article, Mycobacterium, 03 medical and health sciences, chemistry.chemical_compound, Viral Proteins, phage lysis, Bacteriolysis, SDG 3 - Good Health and Well-being, LysB, Cell Wall, Virology, Endopeptidases, 030304 developmental biology, 0303 health sciences, biology, 030306 microbiology, Chemistry, Mycobacterium smegmatis, Hydrolysis, Cell Membrane, Mycobacteria, Phage lysis, Mycobacteriophages, biology.organism_classification, QR1-502, Infectious Diseases, Biochemistry, Lytic cycle, Host cell envelope, mycobacteriophage Ms6, Bacterial outer membrane, Mycobacteriophage Ms6, Protein Binding

Abstract

Double-stranded DNA bacteriophages end their lytic cycle by disrupting the host cell envelope, which allows the release of the virion progeny. Each phage must synthesize lysis proteins that target each cell barrier to phage release. In addition to holins, which permeabilize the cytoplasmic membrane, and endolysins, which disrupt the peptidoglycan (PG), mycobacteriophages synthesize a specific lysis protein, LysB, capable of detaching the outer membrane from the complex cell wall of mycobacteria. The family of LysB proteins is highly diverse, with many members presenting an extended N-terminus. The N-terminal region of mycobacteriophage Ms6 LysB shows structural similarity to the PG-binding domain (PGBD) of the φKZ endolysin. A fusion of this region with enhanced green fluorescent protein (Ms6LysBPGBD-EGFP) was shown to bind to Mycobacterium smegmatis, Mycobacterium vaccae, Mycobacterium bovis BGC and Mycobacterium tuberculosis H37Ra cells pretreated with SDS or Ms6 LysB. In pulldown assays, we demonstrate that Ms6 LysB and Ms6LysBPGBD-EGFP bind to purified peptidoglycan of M. smegmatis, Escherichia coli, Pseudomonas aeruginosa and Bacillus subtilis, demonstrating affinity to PG of the A1γ chemotype. An infection assay with an Ms6 mutant producing a truncated version of LysB lacking the first 90 amino acids resulted in an abrupt lysis. These results clearly demonstrate that the N-terminus of Ms6 LysB binds to the PG.

Published

2021

2. Genome analysis ofSalmonella entericaserovar Typhimurium bacteriophage L, indicator for StySA (StyLT2III) restriction-modification system action

Author

Peter Weigele, Colleen McClung, Sherwood Casjens, Cristian I. Ruse, Graham F. Hatfull, Roger W. Hendrix, Ching-Chung Ko, Julie Zaworski, Robert H. Edgar, and Elisabeth A. Raleigh

Subjects

Bacteriophage, Genetics, biology, Host cell envelope, Restriction modification system, Superinfection exclusion, biology.organism_classification, Gene, Genome, GC-content, Genomic organization

Abstract

Bacteriophage L, a P22-like phage ofSalmonella entericasv Typhimurium LT2, was important for definition of mosaic organization of the lambdoid phage family and for characterization of restriction-modification systems ofSalmonella. We report the complete genome sequences of bacteriophage LcI−4013−am43 and LcII−101; the deduced sequence of wildtype L is 40,633 bp long with a 47.5% GC content. We compare this sequence with those of P22 and ST64T, and predict 71 Coding Sequences, 2 tRNA genes and 14 intergenic rho-independent transcription terminators. The overall genome organization of L agrees with earlier genetic and physical evidence; for example, no secondary immunity region (ImmI:ant,arc) or genes for superinfection exclusion (sieAandsieB) are present. Proteomic analysis confirmed identification of virion proteins, along with low levels of assembly intermediates and host cell envelope proteins. The genome of L is 99.9% identical at the nucleotide level to that reported for phage ST64T, despite isolation on different continents ~35 years apart. DNA modification by the epigenetic regulator Dam is generally incomplete. Dam modification is also selectively missing in one location, corresponding to the P22 phase-variation-sensitive promoter region of the serotype-convertinggtrABCoperon. The number of sites for SenLTIII (StySA) action may account for stronger restriction of L (13 sites) than of P22 (3 sites).

Published

2020

3. Genome analysis of Salmonella enterica serovar Typhimurium bacteriophage L, indicator for StySA (StyLT2III) restriction-modification system action

Author

Robert H. Edgar, Sherwood Casjens, Julie Zaworski, Peter Weigele, Colleen McClung, Roger W. Hendrix, Elisabeth A. Raleigh, Ching-Chung Ko, Cristian I. Ruse, and Graham F. Hatfull

Subjects

Proteomics, Salmonella typhimurium, AcademicSubjects/SCI01140, AcademicSubjects/SCI00010, viruses, restriction indicator, Superinfection exclusion, QH426-470, Serogroup, AcademicSubjects/SCI01180, Genome, Bacteriophage, 03 medical and health sciences, methylation state, Genetics, Bacteriophages, DNA Restriction-Modification Enzymes, Molecular Biology, Gene, Genetics (clinical), 030304 developmental biology, Genomic organization, virion composition, 0303 health sciences, biology, phage tRNA, 030302 biochemistry & molecular biology, biology.organism_classification, Genome Report, lambdoid phage, mosaic genome, Host cell envelope, Restriction modification system, AcademicSubjects/SCI00960, GC-content

Abstract

Bacteriophage L, a P22-like phage of Salmonella enterica sv Typhimurium LT2, was important for definition of mosaic organization of the lambdoid phage family and for characterization of restriction-modification systems of Salmonella. We report the complete genome sequences of bacteriophage L cI–40 13–am43 and L cII–101; the deduced sequence of wildtype L is 40,633 bp long with a 47.5% GC content. We compare this sequence with those of P22 and ST64T, and predict 72 Coding Sequences, 2 tRNA genes and 14 intergenic rho-independent transcription terminators. The overall genome organization of L agrees with earlier genetic and physical evidence; for example, no secondary immunity region (immI: ant, arc) or known genes for superinfection exclusion (sieA and sieB) are present. Proteomic analysis confirmed identification of virion proteins, along with low levels of assembly intermediates and host cell envelope proteins. The genome of L is 99.9% identical at the nucleotide level to that reported for phage ST64T, despite isolation on different continents ∼35 years apart. DNA modification by the epigenetic regulator Dam is generally incomplete. Dam modification is also selectively missing in one location, corresponding to the P22 phase-variation-sensitive promoter region of the serotype-converting gtrABC operon. The number of sites for SenLTIII (StySA) action may account for stronger restriction of L (13 sites) than of P22 (3 sites).

Published

2020

4. Structure and Analysis of R1 and R2 Pyocin Receptor-Binding Fibers

Author

Dean Scholl, Petr G. Leiman, Mikhail M. Shneider, and S.A. Buth

Subjects

Models, Molecular, Protein Conformation, alpha-Helical, 0301 basic medicine, Cell, lcsh:QR1-502, Gene Expression, receptor-binding protein, Crystallography, X-Ray, medicine.disease_cause, lcsh:Microbiology, pseudomonas aeruginosa, Substrate Specificity, R-type pyocin, phage, Magnesium, Cloning, Molecular, Pyocins, pseudomonas-aeruginosa, Chemistry, Depolarization, Recombinant Proteins, 3. Good health, Infectious Diseases, medicine.anatomical_structure, Membrane, Host cell envelope, contractile injection systems, Thermodynamics, short tail fiber, Protein Binding, Viral protein, Iron, Genetic Vectors, 030106 microbiology, bacteriophage k1f, Article, 03 medical and health sciences, Bacteriocin, bacteriocin, Cations, Virology, Escherichia coli, medicine, Protein Interaction Domains and Motifs, Binding site, X-ray crystallography, Binding Sites, model, c-terminal domain, Sodium, crystal-structure, central spike, Pseudomonas aeruginosa, 030104 developmental biology, Cytoplasm, Biophysics, escherichia-coli, Calcium, Protein Conformation, beta-Strand, tailspike protein

Abstract

The R-type pyocins are high-molecular weight bacteriocins produced by some strains of Pseudomonas aeruginosa to specifically kill other strains of the same species. Structurally, the R-type pyocins are similar to &ldquo, simple&rdquo, contractile tails, such as those of phage P2 and Mu. The pyocin recognizes and binds to its target with the help of fibers that emanate from the baseplate structure at one end of the particle. Subsequently, the pyocin contracts its sheath and drives the rigid tube through the host cell envelope. This causes depolarization of the cytoplasmic membrane and cell death. The host cell surface-binding fiber is ~340 &Aring, long and is attached to the baseplate with its N-terminal domain. Here, we report the crystal structures of C-terminal fragments of the R1 and R2 pyocin fibers that comprise the distal, receptor-binding part of the protein. Both proteins are ~240 &Aring, long homotrimers in which slender rod-like domains are interspersed with more globular domains&mdash, two tandem knob domains in the N-terminal part of the fragment and a lectin-like domain at its C-terminus. The putative substrate binding sites are separated by about 100 &Aring, suggesting that binding of the fiber to the cell surface causes the fiber to adopt a certain orientation relative to the baseplate and this then triggers sheath contraction.

Published

2018

5. Molecular and morphological description of Haemoproteus (Parahaemoproteus) bukaka (species nova), a haemosporidian associated with the strictly Australo-Papuan host Subfamily Cracticinae

Author

Robert D. Adlard, William Goulding, Nicholas J. Clark, and Sonya M. Clegg

Subjects

0106 biological sciences, 0301 basic medicine, Zoology, Context (language use), 010603 evolutionary biology, 01 natural sciences, Host-Parasite Interactions, 03 medical and health sciences, parasitic diseases, Animals, Passeriformes, Endemism, Protozoan Infections, Animal, Phylogeny, Islands, General Veterinary, biology, Bird Diseases, General Medicine, Butcherbird, Haemosporida, biology.organism_classification, Cracticus louisiadensis, Honeyeater, 030104 developmental biology, Infectious Diseases, Insect Science, Molecular phylogenetics, Host cell envelope, Parasitology, Haemoproteus

Abstract

Linking morphological studies with molecular phylogeny is important to understanding cryptic speciation and the evolution of host-parasite relationships. Haemosporidian parasites of the Australo-Papuan bird family Artamidae are relatively unstudied. Only one parasite species from the subfamily Cracticinae has been described, and this was based solely on morphological description. This is despite many Cracticinae species being easily observed and abundant over large ranges and in close proximity to human populations. We used morphological and molecular methods to describe a new Haemoproteus species (H. bukaka sp. nov.) from an endemic Butcherbird host (Cracticus louisiadensis) in a relatively unstudied insular area of high avian endemism (Papua New Guinea's Louisiade Archipelago). Phylogenetic reconstructions using parasite cyt-b gene sequences placed the proposed Haemoproteus bukaka sp. nov. close to other host-specialist Haemoproteus species that infect meliphagid honeyeater hosts in the region, e.g. H. ptilotis. Distinct morphological characters of this haemosporidian include macrogametocytes with characteristic large vacuoles opposing a subterminal nucleus on the host cell envelope. Among 27 sampled individuals, prevalence of H. bukaka sp.nov. was high (74 % infection rate) but strongly variable across four islands in the archipelago (ranging from 0 to 100 % prevalence). Parasitaemia levels were low across all infected individuals (0.1-0.6 %). We suspect host density may play a role in maintaining high prevalence given the close proximity and similar physical environments across islands. The findings are discussed in the context of the host genus Cracticus and theory relating to parasite-host evolution and its conservation implications in Papua New Guinea.

Published

2016

6. Structure of a Bacterial Virus DNA-Injection Protein Complex Reveals a Decameric Assembly with a Constricted Molecular Channel

Author

Tsutomu Matsui, Jeffrey A. Speir, Thomas M. Weiss, Lingfei Liang, Haiyan Zhao, Brittany Varnado, Anna Y. Lynn, Liang Tang, and Zihan Lin

Subjects

Models, Molecular, 0301 basic medicine, Phagemid, Cell Membranes, lcsh:Medicine, Biochemistry, Negative Staining, Viral Packaging, Bacteriophage, chemistry.chemical_compound, Protein structure, Macromolecular Structure Analysis, Bacteriophages, lcsh:Science, Staining, Multidisciplinary, Molecular Structure, biology, Physics, Solutions, Nucleic acids, Chemistry, Viruses, Physical Sciences, Host cell envelope, Cellular Structures and Organelles, Cell envelope, Research Article, Protein Structure, Research and Analysis Methods, Microbiology, Viral Proteins, 03 medical and health sciences, Imaging, Three-Dimensional, Virology, Genetics, Molecular Biology, Chemical Physics, Host Cells, lcsh:R, Organisms, Biology and Life Sciences, Proteins, DNA structure, Cell Biology, DNA, biology.organism_classification, Molecular biology, Viral Replication, Protein Structure, Tertiary, 030104 developmental biology, chemistry, Specimen Preparation and Treatment, Cytoplasm, DNA, Viral, Biophysics, lcsh:Q, Protein Multimerization, Bacterial virus, Viral Transmission and Infection

Abstract

The multi-layered cell envelope structure of Gram-negative bacteria represents significant physical and chemical barriers for short-tailed phages to inject phage DNA into the host cytoplasm. Here we show that a DNA-injection protein of bacteriophage Sf6, gp12, forms a 465-kDa, decameric assembly in vitro. The electron microscopic structure of the gp12 assembly shows a ~150-Å, mushroom-like architecture consisting of a crown domain and a tube-like domain, which embraces a 25-Å-wide channel that could precisely accommodate dsDNA. The constricted channel suggests that gp12 mediates rapid, uni-directional injection of phage DNA into host cells by providing a molecular conduit for DNA translocation. The assembly exhibits a 10-fold symmetry, which may be a common feature among DNA-injection proteins of P22-like phages and may suggest a symmetry mismatch with respect to the 6-fold symmetric phage tail. The gp12 monomer is highly flexible in solution, supporting a mechanism for translocation of the protein through the conduit of the phage tail toward the host cell envelope, where it assembles into a DNA-injection device.

Published

2016

7. Structure of phage P22 cell envelope–penetrating needle

Author

Sherwood R. Casjens, Gino Cingolani, and Adam S. Olia

Subjects

Models, Molecular, biology, Protein Conformation, Viral protein, Molecular Sequence Data, Viral Tail Proteins, Crystallography, X-Ray, biology.organism_classification, medicine.disease_cause, Protein Structure, Tertiary, Bacteriophage, Crystallography, Protein structure, Structural Biology, Host cell envelope, medicine, Biophysics, Amino Acid Sequence, Cell envelope, Lipid bilayer, Molecular Biology, Peptide sequence, Bacteriophage P22

Abstract

Bacteriophage P22 infects Salmonella enterica by injecting its genetic material through the cell envelope. During infection, a specialized tail needle, gp26, is injected into the host, likely piercing a hole in the host cell envelope. The 2.1-Å crystal structure of gp26 reveals a 240-Å elongated protein fiber formed by two trimeric coiled-coil domains interrupted by a triple β-helix.The N terminus of gp26 plugs the portal protein channel, retaining the genetic material inside the virion. The C-terminal tip of the fiber exposes β-hairpins with hydrophobic tips similar to those seen in class II fusion peptides. The α-helical core connecting these two functionally polarized tips presents four trimerization octads with consensus sequence IXXLXXXV. The slender conformation of the gp26 fiber minimizes the surface exposed to solvent, which is consistent with the idea that gp26 traverses the cell envelope lipid bilayers.

Published

2007

8. Interaction between the genomes of Lactococcus lactis and phages of the P335 species

Author

Sinead C. Leahy, Suzanne C. Lambie, William J. Kelly, and Eric Altermann

Subjects

Microbiology (medical), cell wall polysaccharides, Lactococcus lactis subsp cremoris, Lactococcus lactis, lcsh:QR1-502, starter culture, Bacterial genome size, Biology, biology.organism_classification, Genome, Microbiology, lcsh:Microbiology, Lytic cycle, Lactococcus lactis subsp. cremoris, Host cell envelope, phage, dairy, Original Research Article, integrase, Gene, genome, Prophage

Abstract

Phages of the P335 species infect Lactococcus lactis and have been particularly studied because of their association with strains of L. lactis subsp. cremoris used as dairy starter cultures. Unlike other lactococcal phages, those of the P335 species may have a temperate or lytic lifestyle, and are believed to originate from the starter cultures themselves. We have sequenced the genome of L. lactis subsp. cremoris KW2 isolated from fermented corn and found that it contains an integrated P335 species prophage. This 41 kb prophage (Φ KW2) has a mosaic structure with functional modules that are highly similar to several other phages of the P335 species associated with dairy starter cultures. Comparison of the genomes of 26 phages of the P335 species, with either a lytic or temperate lifestyle, shows that they can be divided into three groups and that the morphogenesis gene region is the most conserved. Analysis of these phage genomes in conjunction with the genomes of several L. lactis strains shows that prophage insertion is site specific and occurs at seven different chromosomal locations. Exactly how induced or lytic phages of the P335 species interact with carbohydrate cell surface receptors in the host cell envelope remains to be determined. Genes for the biosynthesis of a variable cell surface polysaccharide and for lipoteichoic acids (LTAs) are found in L. lactis and are the main candidates for phage receptors, as the genes for other cell surface carbohydrates have been lost from dairy starter strains. Overall, phages of the P335 species appear to have had only a minor role in the adaptation of L. lactis subsp. cremoris strains to the dairy environment, and instead they appear to be an integral part of the L. lactis chromosome. There remains a great deal to be discovered about their role, and their contribution to the evolution of the bacterial genome.

Published

2013

9. Massive activation of archaeal defense genes during viral infection

Author

Jean-Yves Coppée, Odile Sismeiro, Marleen Voet, Tessa E. F. Quax, John van der Oost, David Prangishvili, Bernd Jagla, Guennadi Sezonov, Marie-Agnès Dillies, Patrick Forterre, Rob Lavigne, Biologie Moléculaire du Gène chez les Extrêmophiles (BMGE), Institut Pasteur [Paris], Transcriptome et Epigénome (PF2), Institut de génétique et microbiologie [Orsay] (IGM), Université Paris-Sud - Paris 11 (UP11)-Centre National de la Recherche Scientifique (CNRS), and Institut Pasteur [Paris] (IP)

Subjects

Gene Expression Regulation, Viral, Immunology, Rudiviridae, Biology, dna, Microbiology, Virus, Host-Parasite Interactions, Sulfolobus, sulfolobus-solfataricus, prokaryotes, 03 medical and health sciences, Microbiologie, Virology, Two-Hybrid System Techniques, CRISPR, [SDV.BBM]Life Sciences [q-bio]/Biochemistry, Molecular Biology, Gene, 030304 developmental biology, VLAG, toxin-antitoxin systems, Regulation of gene expression, Genetics, host interactions, 0303 health sciences, 030306 microbiology, crispr rnas, Archaeal Viruses, Sequence Analysis, DNA, Genome Replication and Regulation of Viral Gene Expression, [SDV.MP]Life Sciences [q-bio]/Microbiology and Parasitology, Lytic cycle, cell-division, differential expression analysis, turreted icosahedral virus, Insect Science, Host cell envelope, Gene Expression Regulation, Archaeal, Transcriptome, complex

Abstract

Archaeal viruses display unusually high genetic and morphological diversity. Studies of these viruses proved to be instrumental for the expansion of knowledge on viral diversity and evolution. The Sulfolobus islandicus rod-shaped virus 2 (SIRV2) is a model to study virus-host interactions in Archaea . It is a lytic virus that exploits a unique egress mechanism based on the formation of remarkable pyramidal structures on the host cell envelope. Using whole-transcriptome sequencing, we present here a global map defining host and viral gene expression during the infection cycle of SIRV2 in its hyperthermophilic host S. islandicus LAL14/1. This information was used, in combination with a yeast two-hybrid analysis of SIRV2 protein interactions, to advance current understanding of viral gene functions. As a consequence of SIRV2 infection, transcription of more than one-third of S. islandicus genes was differentially regulated. While expression of genes involved in cell division decreased, those genes playing a role in antiviral defense were activated on a large scale. Expression of genes belonging to toxin-antitoxin and clustered regularly interspaced short palindromic repeat (CRISPR)-Cas systems was specifically pronounced. The observed different degree of activation of various CRISPR-Cas systems highlights the specialized functions they perform. The information on individual gene expression and activation of antiviral defense systems is expected to aid future studies aimed at detailed understanding of the functions and interplay of these systems in vivo .

Published

2013

10. Structural plasticity of the phage P22 tail needle gp26 probed with xenon gas

Author

Sherwood R. Casjens, Gino Cingolani, and Adam S. Olia

Subjects

Models, Molecular, Xenon, Protein Conformation, Molecular Sequence Data, chemistry.chemical_element, Crystal structure, Biochemistry, Article, Ion, Protein structure, Chlorides, Side chain, Amino Acid Sequence, Molecular Biology, Bacteriophage P22, Mechanical Phenomena, Penetration (firestop), Viral Tail Proteins, Crystallography, chemistry, Host cell envelope, Biophysics, Calcium, Protein Binding

Abstract

The tail needle, gp26, is a highly stable homo-trimeric fiber found in the tail apparatus of bacteriophage P22. In the mature virion, gp26 is responsible for plugging the DNA exit channel, and likely plays an important role in penetrating the host cell envelope. In this article, we have determined the 1.98 A resolution crystal structure of gp26 bound to xenon gas. The structure led us to identify a calcium and a chloride ion intimately bound at the interior of alpha-helical core, as well as seven small cavities occupied by xenon atoms. The two ions engage in buried polar interactions with gp26 side chains that provide specificity and register to gp26 helical core, thus enhancing its stability. Conversely, the distribution of xenon accessible cavities correlates well with the flexibility of the fiber observed in solution and in the crystal structure. We suggest that small internal cavities in gp26 between the helical core and the C-terminal tip allow for flexible swinging of the latter, without affecting the overall stability of the protein. The C-terminal tip may be important in scanning the bacterial surface in search of a cell-envelope penetration site, or for recognition of a yet unidentified receptor on the surface of the host.

Published

2009

11. The small viral membrane-associated protein P32 is involved in bacteriophage PRD1 DNA entry

Author

A. Marika Grahn, Dennis H. Bamford, and Rimantas Daugelavičius

Subjects

Phage display, Genes, Viral, Phagemid, viruses, Immunology, Molecular Sequence Data, Biology, Virus Replication, Microbiology, Permeability, 03 medical and health sciences, chemistry.chemical_compound, Viral Envelope Proteins, Viral entry, Cell Wall, Virology, Gram-Negative Bacteria, Bacteriophage PRD1, Amino Acid Sequence, 030304 developmental biology, 0303 health sciences, 030306 microbiology, Viral membrane, Molecular biology, Cell biology, Virus-Cell Interactions, Molecular Weight, chemistry, Lytic cycle, Insect Science, Host cell cytoplasm, Host cell envelope, DNA, Gene Deletion

Abstract

The lipid-containing bacteriophage PRD1 infects a variety of gram-negative cells by injecting its linear double-stranded DNA genome into the host cell cytoplasm, while the protein capsid is left outside. The virus membrane and several structural proteins are involved in phage DNA entry. In this work we identified a new infectivity protein of PRD1. Disruption of geneXXXIIresulted in a mutant phenotype defective in phage reproduction. The absence of the protein P32 did not compromise the particle assembly but led to a defect in phage DNA injection. In P32-deficient particles the phage membrane is unable to undergo a structural transformation from a spherical to a tubular form. Since P32−particles are able to increase the permeability of the host cell envelope to a degree comparable to that found with wild-type particles, we suggest that the tail-tube formation is needed to eject the DNA from the phage particle rather than to reach the host cell interior.

Published

2002

12. Modification of Escherichia coli membranes in the prereplicative phase of phage T4 infection. Specificity of association and quantitation of bound phage proteins

Author

J P Rosenbusch and B J Takacs

Subjects

Cell Biology, Biology, medicine.disease_cause, Biochemistry, Cell membrane, Membrane, medicine.anatomical_structure, Membrane protein, Lytic cycle, Host cell envelope, medicine, Cell envelope, Bacterial virus, Molecular Biology, Escherichia coli

Abstract

Reinfection of Escherichia coli with the bacterial virus T4 causes modifications of the properties of the host cell envelope during the preeplicative phase of the lytic cycle. These changes include altered densities cell enveloped and their subfractions, morphological modifications of membrane vesicles, and association of newly synthesized proteins with the host cell envelope. Polypeptide analysis by high resolution electrophoresis on polyacrylamide slab gels in dodecyl sulfate revealed that most of some 30 prereplicative phage-coded polypeptides are attached to this structure. Different means of cell disruption and selective extraction procedures, such as variations of ionic strength, removal of divalent cations, and the addition of chaotropic agents or detergents were used to study the characteristics of these attachments. Many proteins appeared to be artifactually absorbed or weakly bound to the envelope, Separation of cell walls from plasma membranes showed that all of the tightly bound proteins were associated withthe cell membrane fraction. The partitioning of phage proteins between the different fractions was monitored using 12 polypeptides which were identified as products of distinct phage genes. Of these, 8 were eliminated as potential membrane markers. Four polypeptides, the products of genes rIIA, rIIB, 39, and 52 were operationally defined as membrane proteins. The number of molecules of the 12 identified phage gene products, synthesized during a single lytic cycle, was determined. The results allowed the estimation of the concentration in the membrane of those proteins which were found to be quantitatively associated with that structure. Association of phage proteins with the cell envelope was found to be unaffected by mutations in any of the identified phage polypeptides.

Published

1975