History of mycoplasma strains and plasmid

screening (XLS

History of mycoplasma strains and plasmid

screening. (XLS 32 KB) Additional file 3: Table S3. Pairwise nucleic sequence identities between mycoplasma plasmids. Global alignments of the full-length nucleic sequence of mycoplasma plasmids were accomplished using a Needleman–Wunsch algorithm implemented in the Needleall program (Needleman & Wunsch, 1970). Identity percents are indicated. Rep group refers to Rep phylogeny (see Figure 6). Table S3. Pairwise nucleic sequence identities between mycoplasma plasmids. Global alignments of the full-length nucleic sequence of mycoplasma plasmids were accomplished using a Needleman–Wunsch algorithm implemented in the Needleall program (Needleman & Wunsch, J Mol Biol 1970;48:443-53). Identity percents are indicated. Rep group refers to Rep phylogeny (see Figure 6). PFT�� in vivo (XLSX 22 KB) Additional file 4: Figure S1. Nucleotide sequences of the predicted ctRNA coding strands. The counter-transcripts were first identified by analogy with those of pMV158 or its derivative pLS1. These ctRNA overlap the rep gene start and have a length of only a few tens of Blasticidin S chemical structure nucleotides. Using the consensus sequence TTGACA – (N17) –TG-N-TATAAT for the promoter, putative promoters were identified in the aligned sequences. Putative Pct promoters are indicated with the -35 and -10 regions in bold and underlined letters. Arrows indicate inverted repeats of the putative rho independent terminators.

The ctRNA of pLS1 (rnaII) is shown as proposed by del Solar et al. [46] with an arrowhead indicating the possible transcriptional Tariquidar datasheet initiation

site. The box CAT indicates the initiation codon of the rep gene that is encoded on the complementary DNA strand. (DOCX 37 KB) Additional file 5: Figure S2. Detection of pMyBK1 ssDNA intermediates Methocarbamol by Southern blot hybridization. Total DNA from Mycoplasma yeatsii type strain GIH TS (lane 1-2) was analyzed on a 0.8% agarose gel (A) with (+) or without (-) prior S1 nuclease treatment. Southern blot (B) was performed with digoxigenin-labeled pMyBK1 probe under non-denaturing conditions. M, DNA ladder. (PPTX 122 KB) Additional file 6: Figure S3. Expression of spiralin in Mcc using pMyBK1 derivatives. Whole cell dot immunoblot of 12 Mcc transformants harboring the spiralin expression vector pCM-K3-spi (a) or the empty vector pCM-K3 (b). Mycoplasma cells were applied to a nitrocellulose membrane and probed with rabbit anti-spiralin antibodies and anti-rabbit IgG peroxidase conjugate. (PPTX 85 KB) References 1. Smets BF, Barkay T: Horizontal gene transfer: perspectives at a crossroads of scientific disciplines. Nature Reviews 2005,3(9):675–678.PubMedCrossRef 2. Frost LS, Leplae R, Summers AO, Toussaint A: Mobile genetic elements: the agents of open source evolution. Nature reviews 2005,3(9):722–732.PubMedCrossRef 3. Razin S, Yogev D, Naot Y: Molecular biology and pathogenicity of mycoplasmas. Microbiol Mol Biol Rev 1998,62(4):1094–1156.PubMed 4.

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