Screening analysis of candidate gene mutations in a kindred with polycystic liver disease

Song Jin; Kai Cui; Zi-Qiang Sun; Yang-Yang Shen; Pang Li; Zhen-Dan Wang; Fei-Fei Li; Ke-Nan Gong; Sheng Li

doi:10.3748/wjg.v21.i8.2343

Screening analysis of candidate gene mutations in a kindred with polycystic liver disease

World J Gastroenterol. 2015 Feb 28;21(8):2343-51. doi: 10.3748/wjg.v21.i8.2343.

Authors

Song Jin¹, Kai Cui¹, Zi-Qiang Sun¹, Yang-Yang Shen¹, Pang Li¹, Zhen-Dan Wang¹, Fei-Fei Li¹, Ke-Nan Gong¹, Sheng Li¹

Affiliation

¹ Song Jin, Zi-Qiang Sun, Department of Hepatobiliary and Vascular Surgery, Affiliated Hospital of Jining Medical College, Jining 272029, Shandong Province, China.

Abstract

Aim: To find potential mutable sites by detecting mutations of the candidate gene in a kindred with polycystic liver disease (PCLD).

Methods: First, we chose a kindred with PCLD and obtained five venous blood samples of this kindred after the family members signed the informed consent form. In the kindred two cases were diagnosed with PCLD, and the left three cases were normal individuals. All the blood samples were preserved at -85 °C. Second, we extracted the genomic DNA from the venous blood samples of the kindred using a QIAamp DNA Mini Kit and then performed long-range polymerase chain reaction (PCR) with different primers. The exons of PKD1 were all sequenced with the forward and reverse primers to ensure the accuracy of the results. Next, we purified the PCR products and directly sequenced them using Big Dye Terminator Chemistry version 3.1. The sequencing reaction was conducted with BiomekFX (Beckman). Finally, we analyzed the results.

Results: A total of 42 normal exons were identified in detecting mutations of the PKD1 gene. A synonymous mutation occurred in exon 5. The mutation was a homozygous T in the proband and was C in the reference sequence. This mutation was located in the third codon and did not change the amino acid encoded by the codon. Missense mutations occurred in exons 11 and 35. These mutations were located in the second codon; they changed the amino acid sequence and existed in the dbSNP library. A nonsense mutation occurred in exon 15. The mutation was a heterozygous CT in the proband and was C in the reference sequence. This mutation was located in the first codon and resulted in a termination codon. This mutation had an obvious influence on the encoded protein and changed the length of the protein from 4303 to 2246 amino acids. This was a new mutation that was not present in the dbSNP library.

Conclusion: The nonsense mutation of exon 15 existed in the proband and in the third individual. Additionally, the proband was heterozygous for this mutation, so the mutable site was a pathogenic mutation.

Keywords: Gene mutation; Kindred; Polycystic liver disease.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Adult
Base Sequence
Codon
Codon, Nonsense*
Cysts / diagnosis
Cysts / genetics*
Cysts / surgery
DNA Mutational Analysis
Exons
Female
Genetic Association Studies
Genetic Markers
Genetic Predisposition to Disease
Heterozygote
Homozygote
Humans
Liver Diseases / diagnosis
Liver Diseases / genetics*
Liver Diseases / surgery
Male
Molecular Sequence Data
Pedigree
Phenotype
TRPP Cation Channels / genetics*
Tomography, X-Ray Computed
Young Adult

Substances

Codon
Codon, Nonsense
Genetic Markers
TRPP Cation Channels
polycystic kidney disease 1 protein

Supplementary concepts

Polycystic liver disease