Cloning and Expression Analysis of Genes Encoding Lytic Endopeptidases L1 and L5 from Lysobacter sp. Strain XL1

Lapteva, Yulia S.; Zolova, O. E.; Shlyapnikov, M. G.; Tsfasman, I. M.; Muranova, T. A.; Stepnaya, O. A.; Kulaev, I. S.; Granovsky, Igor

doi:10.1128/aem.01621-12

Cited by 21 publications

(7 citation statements)

References 46 publications

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“…The phage-related COGs can be further described as follows. Firstly, AlpA is a hydrolase, and its function is to break down the bacterial cell (Lapteva et al, 2012). Secondly, phage endonuclease and primase are essential enzymes for phage DNA replication (Duerkop et al, 2012;Ilyina et al, 1992) and the former can induce the degradation of bacterial genomic DNA (Panayotatos and Fontaine, 1985).…”

Section: Discussionmentioning

confidence: 99%

Bacteriophage of the Skin Microbiome in Patients with Psoriasis and Healthy Family Controls

Wang

Chan

et al. 2020

Journal of Investigative Dermatology

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The bacteriophage (phage) component of the skin microbiome in patients with psoriasis has not been systematically explored. The purpose of this study is to investigate phage and bacterial components of the skin microbiome in patients with psoriasis and in healthy family controls. Lesional skin swabs of four different locations (elbow, forearm, knee, and scalp) were taken from patients with psoriasis. Healthy skin swabs of matched locations were taken from contralateral non-lesional skin and healthy family controls. Skin microbiomes were investigated using next-generation shotgun metagenomics sequencing. 81 skin microbiome samples (27 lesional skin samples and 54 healthy skin samples from contralateral non-lesional skin and family controls) obtained from 16 subjects with psoriasis and 16 matched family controls were sequenced and analyzed. Among phage species with abundant host bacteria, two significantly differential abundant phage species, Acinetobacter phage Presley and Pseudomonas phage O4 (adjusted P < 0.05), between psoriasis lesional skin and healthy skin were identified. Samples with high levels of these phage species had their host bacteria abundance suppressed (P ¼ 0.03 and P < 0.001). Differential phage composition between lesional skin in patients with psoriasis and healthy skin from contralateral non-lesional sites and family controls, as well as the suppression of bacteria host of the respective phage, suggest possible avenues for probiotic phage therapeutics.

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Section: Discussionmentioning

confidence: 99%

Bacteriophage of the Skin Microbiome in Patients with Psoriasis and Healthy Family Controls

Wang

Chan

et al. 2020

Journal of Investigative Dermatology

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“…XL1, with 78% and 58% sequence identity to the L. enzymogenes preproenzyme. 28,29 Another α-lytic protease was purified from the culture medium of Achromobacter lyticus, and N-terminal sequencing/ amino acid compositional analysis of the mature enzyme suggested that large segments are identical to the L. enzymogenes prototype. 30 The A. lyticus α-lytic protease was shown to cleave the N-acetylmuramoyl-l-alanine amide bond and the d-Ala-Gly and Gly-Gly bonds of S. aureus peptidoglycan.…”

Section: Identification Of L Gummosus Proteins Co-purifying With Biomentioning

confidence: 99%

Biofilm-degrading enzymes fromLysobacter gummosus

2014

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Biofilm-degrading enzymes could be used for the gentle cleaning of industrial and medical devices and the manufacture of biofilm-resistant materials. We therefore investigated 20 species and strains of the bacterial genus Lysobacter for their ability to degrade experimental biofilms formed by Staphylococcus epidermidis, a common nosocomial pathogen typically associated with device-related infections. The highest biofilm-degradation activity was achieved by L. gummosus. The corresponding enzymes were identified by sequencing the L. gummosus genome. Partial purification of the biofilm-degrading activity from an extract of extracellular material followed by peptide mass fingerprinting resulted in the identification of two peptidases (α-lytic protease and β-lytic metalloendopeptidase) that were predicted to degrade bacterial cell walls. In addition, we identified two isoforms of a lysyl endopeptidase and an enzyme similar to metalloproteases from Vibrio spp. Potential peptidoglycan-binding C-terminal fragments of two OmpA-like proteins also co-purified with the biofilm-degrading activity. The L. gummosus genome was found to encode five isoenzymes of α-lytic protease and three isoenzymes of lysyl endopeptidase. These results indicated that the extracellular digestion of biofilms by L. gummosus depends on multiple bacteriolytic and proteolytic enzymes, which could now be exploited for biofilm control.

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“…Enzymes L1 and L5 are synthesized in the bacterial cytosol as pre-pro-proteins, which suggests secretion through the cytoplasmic membrane via a Sec-export mechanism [Granovsky et al, 2010[Granovsky et al, , 2011Muranova et al, 2004;Lapteva et al, 2012]. For Lysobacter , there has been no data defining the existence of a similar mechanism.…”

Section: Formation Of Vesicles In Lysobacter Sp and Their Role In Sementioning

confidence: 99%

“…The most investigated among these enzymes are lytic proteases L1 and L5. The gene structures of these proteins ( alp A and alp B) suggest them to be synthesized as pre-pro-proteins, as has been shown for the alpha-lytic protease of Lysobacter enzymogenes , which is homologous to them [Granovsky et al, 2010[Granovsky et al, , 2011Lapteva et al, 2012;Muranova et al, 2004]. In accordance with this, it could be assumed that secretion of enzymes L1 and L5 from the cytosol into the environment should proceed by the same protocol, in two stages.…”

Section: Introductionmentioning

confidence: 99%

The Role of Membrane Vesicles in Secretion of <b><i>Lysobacter</i></b> sp. Bacteriolytic Enzymes

et al. 2013

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Membrane vesicles produced by bacteria have been intensively studied in the recent years. Investigators have noted their roles in essential processes in the bacterial cell including secretion of proteins by the ‘eukaryotic' vesicular mechanism. To date, formation of vesicles is not considered to be a spontaneous event. Many believe it to be a programmed process that can be guided by several mechanisms. Vesicles are derivatives of the cell envelope, which in turn is a supramolecular structure where the functioning and biogenesis of all components are interrelated. Proteins secreted beyond the cell in their translocation are also part of the cell envelope. This also suggests their role in vesicle biogenesis. This review presents the results of vesicle studies in the Gram-negative bacterium Lysobacter sp. This bacterium is of interest as it secretes a number of proteins to the environment, including bacteriolytic enzymes. Bacteriolytic enzymes, on the one hand, are important for studies from a medical point of view as they can form the basis of new generation antimicrobial means. On the other hand, they are a convenient subject for studies of vesicle functions in the vital activities of the bacterial cell.

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Cloning and Expression Analysis of Genes Encoding Lytic Endopeptidases L1 and L5 from Lysobacter sp. Strain XL1

Cited by 21 publications

References 46 publications

Bacteriophage of the Skin Microbiome in Patients with Psoriasis and Healthy Family Controls

Bacteriophage of the Skin Microbiome in Patients with Psoriasis and Healthy Family Controls

Biofilm-degrading enzymes fromLysobacter gummosus

The Role of Membrane Vesicles in Secretion of <b><i>Lysobacter</i></b> sp. Bacteriolytic Enzymes

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