Although a number of enrichment vials were depleted of methyl halides even after as little as 2 weeks of incubation, many of these cultures failed
to degrade a second pulse of methyl halide addition to the headspace. Depletion of methyl halides, accompanied by an optical density (560 nm) of at least 0.4, was used to determine that there had potentially been enrichment of methyl halide-degrading microorganisms. Enrichment cultures that showed successful enrichment of methyl halide-degrading microorganisms are reported in Table 2. Enrichment numbers 165, 165.2, 189, 249 and 273, all cultures initially supplied with formate (10 mM) and methyl bromide (430 μM), degraded between 89 and 268 μmol of methyl bromide. These cultures were subcultured at least twice in fresh 0.1× ANMS medium with 0.2% (v/v) CH3Br in the TSA HDAC ic50 headspace. GC monitoring of these enrichment cultures
was carried out at intervals of approximately 1–2 weeks, meaning that it was not possible to accurately determine the time of depletion of substrate. Generally, initial degradation of methyl halides of these enrichments required at least 1 month, and the time it took to degrade the total amount of methyl halide shown in Table 2 was between 2 and 4 months. Enrichment cultures initially supplied with methanol, methylamine, formate and methane as enrichment substrates were pooled, amended with an additional 0.2% (v/v) headspace CH3Br and subcultured again. This pooled enrichment culture (PE2) also degraded
Ibrutinib mw methyl bromide (580 μmol in total) over the course of 4 months. PCR products generated using the cmuA primer pair from two of these enrichment cultures, the station 8 enrichment (189) and the pooled enrichments (PE2) which had consumed second 89 and 580 μmol of CH3Br, respectively), were cloned as before. An alternative enrichment strategy was used with samples of seawater from L4, a sampling station off the coast of Plymouth. Larger volumes of water unamended with media were incubated with 0.2% (v/v) CH3Br, and the amount of CH3Br consumed was recorded (Table 2). PCR products were obtained from all three enrichment cultures, and one of these, enrichment L4.1, was selected for clone library analysis. The four clone libraries were dereplicated by RFLP, as for the SAP sample libraries, and representative clones were sequenced. Phylogenetic trees of cmuA sequences from all seven libraries were constructed (Fig. 2) and indicated that sequences fell into three major clades with strong nearest neighbour interchange value support. Two of these clades (1 and 3) are novel, with no similar CmuA sequences from extant bacteria. The closest relatives of clade 1 members were cloned cmuA genes from soils and H.