Patent ID: 8945833
Filing Date: 2015-02-03
Classification: C12Q

Abstract:
1. Method for determining drug resistance mutations in any of the non-structural protein regions NS3 to NS5B of Hepatitis C Virus (HCV) for genotypes 1 to 6, more in particular for subtype specific genotypes 1a, 1b, 2a, 2b, 3a, 4a and 4d, present in a sample comprising: a) obtaining said sample from a patient, b) extracting viral genetic material from said sample, c) amplification of the NS5B region of HCV to generate a DNA amplicon of 388 base pairs by using primers having the sequences selected from the group consisting of SEQ ID NO's 1-5, d) sequencing of the amplicon to obtain a sequence of 329 base pairs by using the sequences selected from the group consisting of SEQ ID NO's 3-5, e) performing phylogenetic tree analysis using the 329 base pair sequence information of NS5B to obtain HCV-subtype information in said patient sample, f 1) using subtype-specific primers having the sequences selected from either the group consisting of SEQ ID NO's 6-9, 42-45, 104-107, 120-123, 145-148 or 180-183 for the generation of a DNA amplicon comprising the non-structural protein NS3 (N-terminal 181 amino acids), g 1) sequencing the NS3 amplicon to obtain a sequence of 543 base pairs by using the sequences selected from the group consisting of SEQ ID NO's 8 and 9; 43 and 45-46; 104 and 106; 120 and 122; 146 and 148 or 180 and 182 h) aligning the sequence obtained in step (g 1), (g 2), (g 3) or (g 4) with a reference or wild-type HCV sequence, i) determining drug resistance mutation(s) in the viral genetic material present in patient sample, j) generating a NS3 amplicon starting from the DNA amplicon comprising the NS3 (N-terminal 181 amino acids) as obtained in step (f 1) using primers having the sequence of SEQ ID NO 11 and 12, k) inserting, by InFusion™ cloning or in vitro recombination, said amplicon obtained in step (i) into a NS3 deleted replication incompetent marker containing shuttle vector having the sequence of SEQ ID NO 10 to obtain a NS3 replication competent recombinant HCV replicon, l) generating RNA, by in vitro transcription, from said HCV replicon obtained in step (k) m) transfecting said RNA into suitable cells, n) determining, based on the expression of the marker gene, the EC