Alignment of five amino acid sequences including LAF 0141, LAF 0655 and other reported NTDs (Fig. 1) showed that, in addition to the three critical catalytic sites for 2′-deoxyribosyl transfer activity (Armstrong

et al., 1996; Anand et al., 2004; Miyamoto et al., 2007), the LAF 0141 gene encodes a LBH589 price substrate binding site that interacts with both purine and pyrimidine bases of 2′-deoxyribonucleosides (Miyamoto et al., 2007). This made LAF 0141 a perfect candidate as an NTD despite the fact that protein sequence identity between LAF 0141 and known NTDs (Kaminski et al., 2008) was only 34%. The LAF 0141 homolog from L. fermentum CGMCC 1.2133 was amplified using PCR, cloned, and overexpressed in E. coli BL21. The recombinant plasmid was sequenced and there were no differences

at the nucleotide level between LAF 0141 and the homolog. To identify the function of the LAF 0141 homolog gene product, the recombinant protein was purified by a combination of two ion-exchange chromatography steps and further via a gel filtration column (Fig. 2a). Purified recombinant LAF learn more 0141 homolog gene product migrated as an 18-kDa protein on 12.5% SDS-PAGE, which was identical with the theoretic molecular mass of 18.28 kDa (a total of 160 amino acids, with two additional amino acids present at the N-terminus). The concentration of the purified protein was 2.9 mg mL−1. The N-deoxyribosyltransferase activity of the purified recombinant protein was determined by reactions between adenine and thymidine under standard conditions. The amount of deoxyribose transferred after GBA3 30 min in citrate buffer was 73.3%. The control reaction, which did not contain the enzyme, showed no conversion of the substrate to a product (Fig. 2b). As PTDs can only catalyze deoxyribosyl transfer to and from purines, and the nucleoside phosphorylases require inorganic phosphates for their enzyme reactions, the LAF 0141 homolog gene product should be classified as an NTD. Subcellular localization of the NTD was determined using the polyclonal antibodies raised against

recombinant NTD. The specificity of the purified antibodies was confirmed using whole cell extract of L. fermentum in Western blotting (Fig. 3a). The bacterial cells were separated into their different compartments, and NTD was detected both in the cytoplasmic fraction and the cell wall/plasma membrane fractions (Fig. 3b). Washing the debris with buffer could exclude possible contamination with cytoplasmic proteins. However, after two washes, NTD signal remains detectable in the washing supernatant indicating that the cell wall/plasma associated NTD might be washed off by the buffer. Immunogold labeling of NTD on ultrathin sections of lactobacilli cells was clearly visualized under the electron microscope, whereas background labeling was relatively low (Fig. 4). The electron-transparent granules can be inferred to be PHB (polyhydroxybutyrate) granules (data not shown).