Whole exome sequencing for diagnosis of hereditary thrombocytopenia

• Published in: Medicine (Baltimore) Vol. 99; no. 47; p. e23275
• Main Authors: Mekchay, Ponthip, Ittiwut, Chupong, Ittiwut, Rungnapa, Akkawat, Benjaporn, Le Grand, Supang Maneesri, Leela-Adisorn, Netchanok, Muanpetch, Suwanna, Khovidhunkit, Weerapan, Sosothikul, Darintr, Shotelersuk, Vorasuk, Suphapeetiporn, Kanya, Rojnuckarin, Ponlapat
• Format: Journal Article
• Language: English
• Published: United States Lippincott Williams & Wilkins 20.11.2020
• Subjects: Adolescent; Adult; Cross-Sectional Studies; Female; Humans; Middle Aged; Mutation; Observational Study; Thrombocytopenia - diagnosis; Thrombocytopenia - genetics; Whole Exome Sequencing; Young Adult
• ISSN: 0025-7974; 1536-5964
• DOI: 10.1097/MD.0000000000023275

Hereditary thrombocytopenia comprises extremely diverse diseases that are difficult to diagnose by phenotypes alone. Definite diagnoses are helpful for patient (Pt) management.To evaluate the role of whole exome sequencing (WES) in these Pts.Cases with unexplained long-standing thrombocytopenia and/or suggestive features were enrolled to the observational study. Bleeding scores and blood smear were evaluated. The variant pathogenicity from WES was determined by bioinformatics combined with all other information including platelet aggregometry, flow cytometry, and electron microscopy (EM).Seven unrelated Pts were recruited. All were female with macrothrombocytopenia. Clinical bleeding was presented in four Pts; extra-hematological features were minimal and family history was negative in every Pt. WES successfully identified all the 11 responsible mutant alleles; of these, four have never been previously reported. Pt 1 with GNE-related thrombocytopenia showed reduced lectin binding by flow cytometry, increased glycogen granules by EM and a novel homozygous mutation in GNE. Pts 2 and 3 had phenotypic diagnoses of Bernard Soulier syndrome and novel homozygous mutations in GP1BB and GP1BA, respectively. Pt 4 had impaired microtubule structures, concomitant delta storage pool disease by EM and a novel heterozygous TUBB1 mutation. Pt 5 had sitosterolemia showing platelets with reduced ristocetin responses and a dilated membrane system on EM with compound heterozygous ABCG5 mutations. Pts 6 and 7 had MYH9 disorders with heterozygous mutations in MYH9.This study substantiates the benefits of WES in identifying underlying mutations of macrothrombocytopenia, expands mutational spectra of four genes, and provides detailed clinical features for further phenotype-genotype correlations.