20-bp DNA ladder was bought from TaKaRa Bio (Dalian, China) Co ,

20-bp DNA ladder was bought from TaKaRa Bio (Dalian, China) Co., Ltd. Goat anti-human IgG-horseradish peroxidase (HRP) was from Jackson ImmunoResearch (Pennsylvania, USA), and goat anti-rabbit IgG-HRP was bought from Santa Cruz (California, USA). UltraEAL Western Blot Detection System was purchased from Shanghai Generay Biotech Co., Ltd (Shanghai, China). Protein molecular weight marker, lymphocyte

separation medium (mouse), mitomycin and CCK-8 kit were purchased from Beyotime Institute of Biotechnology (Jiangsu, China). ELISA kits for IFN-γ or IL-4 were purchased from R&D Systems (Minnesota, USA). Sera from L. interrogans, recombinant protein OmpL1- or LipL41-immunized rabbits PF-562271 cost were produced as previously described [17, 18]. Sera of leptospirosis patients were obtained from hospitals in Guangdong, Sichuan and Zhejiang Fluorouracil provinces [19]. 6-8 week old female BALB/c mice were procured from the Experimental Animal Center of Zhejiang University and raised under pathogen-free environment. All the animal experiments were approved by the institutional review board. Prediction of T and B cell epitopes The combined T and B cell epitopes were predicted based on the amino acid sequences of OmpL1 and LipL41 (GenBank accession codes AAT48511

and AAT48493). To avoid the epitopes located in the signal peptide region, SignalP 3.0 Server (http://​www.​cbs.​dtu.​dk/​services/​SignalP/​) was used to predict the signal peptides. ANTIGENIC program in EMBOSS (http://​beta.​immuneepitope.​org/​) was used to predict B cell epitopes and ProPred, a web tool useful in the prediction of HLA-DR binding sites (http://​www.​imtech.​res.​in/​raghava/​hlapred/​) [20], was used to predict potential T cell epitopes. Extraction of genomic DNA The genomic DNA of L. interrogans Lai strain Acesulfame Potassium was extracted by proteinase K treatment and phenol-chloroform extraction method as described previously [21]. The precipitated genomic DNA was resuspended in 100 μl sterilized water, 10 μl 3 M sodium acetate and 220 μl absolute alcohol and stored at -20°C. Before use, DNA was precipitated by centrifugation and was resuspended in sterilized water. Expression and purification of

epitope peptides Sequences of 4 predicted epitopes from OmpL1 and 4 from LipL41 were amplified from genomic DNA. The primers used to amplify the fragments of selected epitopes were shown in Table 1. Eco R52 I site and a 14 bp leader peptide sequence of M13KE were located at the 5′ end of each forward primer, and Kpn I was introduced at the 5′ end of reverse primer. The amplified fragments were inserted into pGEM-T easy vector for sequencing. Then each of the sequence-confirmed fragment was subcloned into Eco R52 I and Kpn I sites of the phage vector M13KE. Primers M13PF 5′-GAGATTTTCAACGTGAAAAAATTATT-3′ and M13PR 5′-TGAATTT TCTGTATGGGATTTTGCTA-3′ were designed based on the sequence of PIII gene in M13KE and were used to determine the insertions of each epitope by colony PCR.

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