We have previously shown [5, 19, 21] that Streptomyces sp. AcH 505 is a fungus-specific MHB that produces

fungus growth regulators and affects plant health and development. When tree roots were inoculated with a suspension of AcH 505 mycelia, significant stimulation of mycorrhiza formation was observed [19]. In the oak system, we also could find a slight increase in the number of mycorrhizas when the microcosm soil was inoculated with AcH 505. This was the first time when the mycorrhization helper effect was observed for AcH 505 in a soil based culture system. The present study further demonstrates the potential of this strain selleck kinase inhibitor by casting light on its performance in a soil-vermiculate formulation, and shows that AcH 505 benefits from the presence of the mycorrhizal fungus. Specific detection of Streptomyces sp. AcH 505 Our initial experiments with AcH 505 were conducted using primers designed against the 16S-23S ribosomal DNA intergenic spacers and single copy genes. However, only the primers targeting the intergenic regions between protein-coding genes yielded specific amplification; the other tested primers were not suitable due to non-specific background amplification when used with samples that included soil microbe DNA. The ribosomal operon is present in

multiple copies in streptomycetes [32], and buy Idasanutlin different species within this genus can have different rDNA copy numbers. Thalidomide Moreover, the rate of rDNA sequence variation between the genomes of different Streptomyces strains is unknown. According to our preliminary analysis of the AcH 505 genome, the intergenic region between the gyrA and gyrB genes exists in a single copy and is thus an excellent target

for specific quantification. The number of available genome data for different Streptomyces strains is increasing [33] and will enable the application of this simple and specific qPCR method for streptomycete Selleckchem A-1210477 quantification for even more bacterial isolates in the future. Comparable detection and quantification of Piloderma croceum by qPCR using two primer pairs In basidiomycete fungi, the ribosomal genes are also present in multiple copies, and changes in the numbers of rRNA genes occur throughout the fungal life cycle [34]. Regions of rDNA are distributed as large tandem arrays, and intra-genomic variation in the length and the base distribution of rDNA sequences has been described [35]. Most qPCR quantification approaches in fungi are based on the internal transcribed spacer regions (ITS1 and ITS2) of the rDNA, since these are easily accessible by PCR and with their high copy number they allow a sensitive detection [27, 28, 31]. Due to the methodological constraints listed above, it can be argued that the use of single copy genes or intergenic regions between protein coding genes could allow for more accurate quantification of basidiomycete fungi. Our observations with P.