Publication:
Molecular analysis of the iduronate-2-sulfatase gene in Thai patients with Hunter syndrome

1

Issued Date

2008-01-01

Resource Type

Article

ISSN

15732665
01418955

DOI

10.1007/s10545-008-0876-z

Other identifier(s)

2-s2.0-84855585793

Rights

Mahidol University

Rights Holder(s)

SCOPUS

Bibliographic Citation

Journal of Inherited Metabolic Disease. Vol.31, No.SUPPL. 2 (2008)

Suggested Citation

S. Keeratichamroen, J. R Ketudat Cairns, D. Wattanasirichaigoon, P. Wasant, L. Ngiwsara, P. Suwannarat, S. Pangkanon, J. Kuptanon, P. Tanpaiboon, T. Rujirawat, S. Liammongkolkul, J. Svasti Molecular analysis of the iduronate-2-sulfatase gene in Thai patients with Hunter syndrome. Journal of Inherited Metabolic Disease. Vol.31, No.SUPPL. 2 (2008). doi:10.1007/s10545-008-0876-z Retrieved from: https://repository.li.mahidol.ac.th/handle/123456789/19012

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Title

Molecular analysis of the iduronate-2-sulfatase gene in Thai patients with Hunter syndrome

Author(s)

S. Keeratichamroen
 J. R Ketudat Cairns
 D. Wattanasirichaigoon
 P. Wasant
 L. Ngiwsara
 P. Suwannarat
 S. Pangkanon
 J. Kuptanon
 P. Tanpaiboon
 T. Rujirawat
 S. Liammongkolkul
 J. Svasti

Other Contributor(s)

Chulabhorn Research Institute
 Suranaree University of Technology
 Mahidol University
 Queen Sirikit National Institute of Child Health
 Chiang Mai University

Abstract

Molecular defects in the gene encoding the enzyme iduronate-2-sulfatase (IDS) result in Hunter disease (mucopolysaccharidosis type II, MPS II). To determine the molecular basis of MPS II in Thailand, the IDS gene was analysed in 20 Thai patients with Hunter syndrome from 18 unrelated families. A total of 19 different mutations, including 9 missense mutations, 3 nonsense mutations, 3 splice site alterations, 1 deletion, 2 indels, and 1 rearrangement were identified, 8 of which were novel (p.R101C, p.D148V, p.G224A, p.K227E, p.E254X, p.W337X, c.440-442delinsTT and c.720-731delinsTTTCAGATGTTCTCCCCAG). Evaluation of the IDS activity of two hemizygous variants identified in the same patient, p.R101C and p.R468Q, by expression of IDS with the individual mutations in COS 7 cells indicated that only the p.R468Q mutation affected IDS protein activity. Two exonic mutations, c.257C>T (p.P86L) and c.418G>A, were found to activate multiple cryptic splice sites, resulting in aberrantly spliced transcripts. Thus, MPS II in Thailand is caused by a diverse set of defects affecting both IDS protein production and activity. © SSIEM and Springer 2008.

Keyword(s)

Biochemistry, Genetics and Molecular Biology
 Medicine

Availability

URI

https://repository.li.mahidol.ac.th/handle/123456789/19012

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