4-21 NP Healthy nt AAZJ00000000 Yes 3655 MEE AOM nt AAZF00000000

4-21 NP Healthy nt AAZJ00000000 Yes 3655 MEE AOM nt AAZF00000000 No 6P18H1 Adult COPD nt AAWW00000000 No Selleck MM-102 7P49H1 Adult COPD nt AAWV00000000 Yes PittAA MEE COM nt AAZG00000000 Yes PittHH MEE COM nt AAZH00000000

No PittII MEE COM nt AAZI00000000 No R2866 BLD nt AADP00000000 No R3021 NP Healthy nt AAZE00000000 Yes 10810 Meningitis b na No F3031 BPF Clone aegyptius na No F3047 BPF Clone aegyptius na No a Site and/or disease state from which strain isolated; NP, nasopharynx, AOM, acute otitis media; MEE, middle ear effusion; COM, chronic otitis media; Ext. Ear Ott, Isolate from external ear in patient with ottorhea; Healthy, Healthy child; COPD, chronic obstructive pulmonary disease; Selleckchem Adavosertib BLD, blood. No source is given for Rd KW20 since this a laboratory strain that has been passaged multiple times since its original isolation [63, 74, 75]. b nt, nontypeable strain; b, type b strain; aegyptius, H. influenzae biogroup aegyptius. c GenBank Accession Numbers

beginning with L or C denote completed genomic sequence, those beginning with AA denote sequences in process of assembly. na, not available (no GenBank accession numbers are available, sequences are accessible at the Wellcome Trust Sanger Institute [43]). d Yes, fhu locus is present; No, fhu locus is absent. As is the case for NTHi strain R2846, none of the H. influenzae INCB024360 solubility dmso genomic sequences analyzed above contained genes with homology to known siderophore biosynthetic genes. In addition to the above in silico analyses of sequenced H. influenzae genomes a PCR based survey of selected strains from a laboratory collection of H. influenzae isolates which had been previously characterized by the electrophoretic mobility of 15 metabolic

enzymes [45] was performed. Thirty-nine strains representing 39 different electrophoretic types (ETs) were used in this study; four of these strains were type b strains and 35 were serologically nontypeable. In addition to characterization by ET these strains were previously characterized by biotype, and representative Non-specific serine/threonine protein kinase strains of each of the five biotypes were analyzed (Table 2). PCR assays for the presence of each gene in the fhu locus in each strain were repeated at least twice. Of the four type b strains tested, none were positive for the presence of any gene in the fhu locus (Table 2). In considering strains by biotype, all of the tested strains of biotypes I, IV and V were negative for the presence of all genes in the fhu locus (Table 2). Of six strains of biotype II, one strain (HI1374) was positive for the presence of fhuCDB and r2846.1777 but was negative for the presence of orf5 (although in at least one of several separate assays the orf5 primers were weakly positive with strain HI1374). Of 21 strains of biotype III, six strains were consistently positive for the presence of all five genes, ten strains were positive for the presence of at least four genes, and one strain (HI1389) was consistently positive for the presence of three genes.

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