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Tion within self-segregating regions known as lipid raft buy PS-1145 microdomains [35,36]. When compared to the surrounding phospholipid membrane, also known as the liquid disordered phase (Ld), lipid rafts typically contain a higher concentration of sphingolipids intercalated with cholesterol [35,36]. Numerous studies suggest that the segregation of lipid raft microdomains from the surrounding bilayer functions to compartmentalize or concentrate specific proteins in order to perform cellular functions, including endocytosis and intracellular signaling by second messenger pathways [37?0]. Since cholesterol serves as the initial binding target for Ply, it is hypothesized that Ply will localize and interact with lipid raft microdomains on the host cell surface. Table 1. Oligonucleotide Primers for Mutagenesis.Furthermore, lipid rafts may function to congregate Ply monomers and increase the probability of oligomerization. Traditionally, the Ply mechanism of action has been studied using either human red blood cells or synthetic membranes, but Ply has never been examined using cells of the human corneal epithelium, which are an example of a cell that is directly and measurably affected by Ply during the course of an infection. Investigating the lytic mechanism of Ply in the context of ocular pathogenesis could lead to the development of targeted treatments that aim to prevent the pathology caused by Ply during pneumococcal keratitis.Materials and Methods Structural DiagramsPly structural cartoons were generated using MacPyMOL version 1.3 based on the primary sequence of Ply from the S. pneumoniae D39 genome (GenBank Accession Number CP000410.1).Plasmids, Bacterial Licochalcone-A Strains, and Cell Growth ConditionsThe wild-type ply gene (plyWT) was amplified from the chromosomal DNA of S. pneumoniae D39, and 11967625 cloned into the pET101D expression vector (Invitrogen, Carlsbad, CA) as previously described and was subsequently named pET101DplyWT [41]. All recombinant Ply expression vectors were transformed in Escherichia coli BL21, and grown at 37uC with aeration at 200 rpm in Luria-Bertani medium (LB) containing 50 mg/ml carbenicillin. Human corneal epithelial cells (HCECs) were a kind gift from Dr. Haydee Bazan (Louisiana State University Eye Center, New Orleans, LA) and were originally established by Dr. Roger Beuerman (Singapore Eye Research Institute). The first use of the HCEC line was described by Sharma et al. in 2003 [42]. HCECsPrimer 1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 PlyA370GSequence (59?9) For ctgctggatcatagtggtggctatgttgcccaa accactatgatccagcagtaaatctccgtttct ctgctggatcatagtggtgaatatgttgcccaa accactatgatccagcagtaaatctccgtttct ggcaggatttgacgggtcactttaccactag ctagtggtaaagtgacccgtcaaatcctgcc ggcaggatttgacggagcactttaccactag ctagtggtaaagtgctccgtcaaatcctgcc gagtgtaccgggcttgccggggaatggtggcgt ggcaagcccggtacactctctaattttgac gagtgtaccgggcttgccgaggaatggtggcgt ggcaagcccggtacactctctaattttgac gagtgtaccgggcttgccttcgaatggtggcgt ggcaagcccggtacactctctaattttgac tctatttggggaacaactggctatcctcaggta agttgttccccaaatagaaatcgtccgctt tctatttggggaacaactgaatatcctcaggta agttgttccccaaatagaaatcgtccgcttStudy This Study This Study This Study This Study This Study This Study This Study This Study This Study This Study This Study This Study Thornton and McDaniel, 2005 [41] Thornton and McDaniel, 2005 [41] This Study This Study This Study This StudyPlyA370G Rev PlyA370E For PlyA370E Rev PlyA406G For PlyA406G Rev PlyA406E For PlyA406E Rev PlyW433G For PlyW433G Rev PlyW433E For PlyW433E Rev.Tion within self-segregating regions known as lipid raft microdomains [35,36]. When compared to the surrounding phospholipid membrane, also known as the liquid disordered phase (Ld), lipid rafts typically contain a higher concentration of sphingolipids intercalated with cholesterol [35,36]. Numerous studies suggest that the segregation of lipid raft microdomains from the surrounding bilayer functions to compartmentalize or concentrate specific proteins in order to perform cellular functions, including endocytosis and intracellular signaling by second messenger pathways [37?0]. Since cholesterol serves as the initial binding target for Ply, it is hypothesized that Ply will localize and interact with lipid raft microdomains on the host cell surface. Table 1. Oligonucleotide Primers for Mutagenesis.Furthermore, lipid rafts may function to congregate Ply monomers and increase the probability of oligomerization. Traditionally, the Ply mechanism of action has been studied using either human red blood cells or synthetic membranes, but Ply has never been examined using cells of the human corneal epithelium, which are an example of a cell that is directly and measurably affected by Ply during the course of an infection. Investigating the lytic mechanism of Ply in the context of ocular pathogenesis could lead to the development of targeted treatments that aim to prevent the pathology caused by Ply during pneumococcal keratitis.Materials and Methods Structural DiagramsPly structural cartoons were generated using MacPyMOL version 1.3 based on the primary sequence of Ply from the S. pneumoniae D39 genome (GenBank Accession Number CP000410.1).Plasmids, Bacterial Strains, and Cell Growth ConditionsThe wild-type ply gene (plyWT) was amplified from the chromosomal DNA of S. pneumoniae D39, and 11967625 cloned into the pET101D expression vector (Invitrogen, Carlsbad, CA) as previously described and was subsequently named pET101DplyWT [41]. All recombinant Ply expression vectors were transformed in Escherichia coli BL21, and grown at 37uC with aeration at 200 rpm in Luria-Bertani medium (LB) containing 50 mg/ml carbenicillin. Human corneal epithelial cells (HCECs) were a kind gift from Dr. Haydee Bazan (Louisiana State University Eye Center, New Orleans, LA) and were originally established by Dr. Roger Beuerman (Singapore Eye Research Institute). The first use of the HCEC line was described by Sharma et al. in 2003 [42]. HCECsPrimer 1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 PlyA370GSequence (59?9) For ctgctggatcatagtggtggctatgttgcccaa accactatgatccagcagtaaatctccgtttct ctgctggatcatagtggtgaatatgttgcccaa accactatgatccagcagtaaatctccgtttct ggcaggatttgacgggtcactttaccactag ctagtggtaaagtgacccgtcaaatcctgcc ggcaggatttgacggagcactttaccactag ctagtggtaaagtgctccgtcaaatcctgcc gagtgtaccgggcttgccggggaatggtggcgt ggcaagcccggtacactctctaattttgac gagtgtaccgggcttgccgaggaatggtggcgt ggcaagcccggtacactctctaattttgac gagtgtaccgggcttgccttcgaatggtggcgt ggcaagcccggtacactctctaattttgac tctatttggggaacaactggctatcctcaggta agttgttccccaaatagaaatcgtccgctt tctatttggggaacaactgaatatcctcaggta agttgttccccaaatagaaatcgtccgcttStudy This Study This Study This Study This Study This Study This Study This Study This Study This Study This Study This Study This Study Thornton and McDaniel, 2005 [41] Thornton and McDaniel, 2005 [41] This Study This Study This Study This StudyPlyA370G Rev PlyA370E For PlyA370E Rev PlyA406G For PlyA406G Rev PlyA406E For PlyA406E Rev PlyW433G For PlyW433G Rev PlyW433E For PlyW433E Rev.

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Author: DNA_ Alkylatingdna