Open AccessCarrier Detection in Glanzmann Thrombasthenia
Author(s) -
Meganathan Kannan,
Firdos Ahmad,
Birendra Kumar Yadav,
Pratik Kumar,
Paresh Jain,
Rajive Kumar,
Renu Saxena
Publication year - 2008
Publication title -
american journal of clinical pathology
Language(s) - Uncategorized
Resource type - Journals
SCImago Journal Rank - 0.859
H-Index - 128
eISSN - 1943-7722
pISSN - 0002-9173
DOI - 10.1309/hye4ap9961cep0c0
Subject(s) - flow cytometry , thrombasthenia , glanzmann's thrombasthenia , western blot , southern blot , microbiology and biotechnology , blot , cytometry , biology , platelet membrane glycoprotein , genetics , gene , immunology , platelet , glycoprotein , platelet aggregation
We studied 20 families with Glanzmann thrombasthenia, including 20 parents and 22 siblings, for carrier detection. Carrier detection was done by phenotypic analysis (flow cytometry and Western blot) and direct gene analysis (sequencing or restriction fragment length polymorphism). Reduced expression of the glycoprotein IIb/IIIa complex was found by flow cytometry in 17 (85%) of the parents and 12 (55%) of the siblings. Western blot showed a reduced or an abnormal band in 6 (30%) of the parents and 8 (36%) of the siblings. DNA analysis in family members showed all parents and 16 (73%) of siblings to be carriers. Both techniques, flow cytometry and Western blot, were evaluated with respect to DNA analysis as a "gold standard" method. The sensitivity of flow cytometry was higher (75%) than that of Western blot (39%). We concluded that flow cytometry can effectively be used for carrier detection in Glanzmann thrombasthenia.
Accelerating Research
Robert Robinson Avenue,
Oxford Science Park, Oxford
OX4 4GP, United Kingdom
Address
John Eccles HouseRobert Robinson Avenue,
Oxford Science Park, Oxford
OX4 4GP, United Kingdom