Your search keyword '"Shane Grimsley"' showing total 3 results

1. Characterization of GYP*Mur and novel GYP*Bun ‐like hybrids in Thai blood donors reveals a qualitatively altered s antigen

Author

Janine Robb, Philaiphon Jongruamklang, Martin L. Olsson, Jill R. Storry, Nicole Thornton, and Shane Grimsley

Subjects

medicine.medical_specialty, Blood Donors, 030204 cardiovascular system & hematology, Compound heterozygosity, 03 medical and health sciences, 0302 clinical medicine, Antigen, Gene Duplication, Internal medicine, Genotype, medicine, Humans, Glycophorin, Glycophorins, Allele, Alleles, Hematology, biology, GYPB, Heterozygote advantage, Sequence Analysis, DNA, General Medicine, Thailand, Molecular biology, Mutation, Blood Group Antigens, biology.protein, 030215 immunology

Abstract

Background and objectives: The Mi(a+) GP(B-A-B) hybrid phenotypes occur with a prevalence of 2%–23% across Southeast Asia. While the s antigen is alleged to be altered, no evidence for specific variants is known. Screening using a monoclonal IgM anti-s mistyped six S‒s+ RBC units as S‒s‒. Further, alloanti-s was identified in an S+s+ patient. Our objective was to investigate the s antigen further. Materials and methods: DNA from 63 Thai blood donor samples PCR-positive for a GYP(B-A-B) hybrid was sequenced with primers spanning GYPB exons 3–4. Flow cytometry was used for semiquantitative analysis of s expression and correlated with the glycophorin genotype. Results: DNA sequencing showed that GYP*Mur was carried by 56/63 samples (88·9%) of which 5/56 lacked normal GYPB: three of these were GYP*Mur homozygotes, one was a compound heterozygote carrying GYP*Mur and a GYP*Bun-like allele (designated GYP*Thai), and the fifth sample carried GYP*Mur and another GYP*Bun-like allele. Seven samples (7/63) were GYP*Thai heterozygotes. IgM monoclonal anti-s (P3BER) did not react with the s antigen carried by GP.Mur or GP.Bun, whereas two IgG anti-s showed enhanced reactivity. Conclusions: We confirmed that GYP*Mur is the most frequent variant in Thai blood donors and also identified GYP*Thai with a frequency of 1·1%. We showed that s antigen on Mi(a+) GP(B-A-B) hybrids is qualitatively altered and should be considered when selecting reagents for phenotyping where such hybrids are prevalent, endemically and in blood centres worldwide. (Less)

Published

2020

2. Development and validation of a universal blood donor genotyping platform: A multinational prospective study

Author

Augusto Rendon, John M. Jongerius, Nicholas A. Watkins, Kim Brügger, Nicholas Gleadall, Daniel Duarte, Tiffany C. Timmer, Sara Trompeter, Matthew R. Walker, Jennifer G. Sambrook, David J. Roberts, Christopher J. Penkett, Carolin M. Sauer, Nieke van der Bolt, Barbera Veldhuisen, Shane Grimsley, Colin Brown, Adam S. Butterworth, Michael J. Sweeting, Salih Tuna, Emanuele Di Angelantonio, John Ord, Karyn Megy, Jessie S Luken, C. Ellen van der Schoot, Ilenia Simeoni, Gail Miflin, William J. Lane, Nicole Thornton, Ram Varma, William J. Astle, Connie M. Westhoff, Christopher S. Nelson, Katja van den Hurk, Jeremy Gollub, Kathleen Stirrups, Willem H. Ouwehand, Femmeke J. Prinsze, Alexander T. Dilthey, John Danesh, Public and occupational health, Graduate School, AII - Inflammatory diseases, APH - Methodology, and Landsteiner Laboratory

Subjects

medicine.medical_specialty, Blood transfusion, Genotype, medicine.medical_treatment, Concordance, Blood Donors, Human leukocyte antigen, 030204 cardiovascular system & hematology, 03 medical and health sciences, 0302 clinical medicine, Isoantibodies, medicine, Humans, Blood Transfusion, Prospective Studies, Typing, Genotyping, biology, Transfusion Medicine, business.industry, Transfusion medicine, Hematology, Biobank, Immunology, biology.protein, Antibody, business, 030215 immunology

Abstract

Each year, blood transfusions save millions of lives. However, under current blood-matching practices, sensitization to non–self-antigens is an unavoidable adverse side effect of transfusion. We describe a universal donor typing platform that could be adopted by blood services worldwide to facilitate a universal extended blood-matching policy and reduce sensitization rates. This DNA-based test is capable of simultaneously typing most clinically relevant red blood cell (RBC), human platelet (HPA), and human leukocyte (HLA) antigens. Validation was performed, using samples from 7927 European, 27 South Asian, 21 East Asian, and 9 African blood donors enrolled in 2 national biobanks. We illustrated the usefulness of the platform by analyzing antibody data from patients sensitized with multiple RBC alloantibodies. Genotyping results demonstrated concordance of 99.91%, 99.97%, and 99.03% with RBC, HPA, and HLA clinically validated typing results in 89 371, 3016, and 9289 comparisons, respectively. Genotyping increased the total number of antigen typing results available from 110 980 to >1 200 000. Dense donor typing allowed identification of 2 to 6 times more compatible donors to serve 3146 patients with multiple RBC alloantibodies, providing at least 1 match for 176 individuals for whom previously no blood could be found among the same donors. This genotyping technology is already being used to type thousands of donors taking part in national genotyping studies. Extraction of dense antigen-typing data from these cohorts provides blood supply organizations with the opportunity to implement a policy of genomics-based precision matching of blood.

Published

2020

3. Lack of the nucleoside transporter ENT1 results in the Augustine-null blood type and ectopic mineralization

Author

Jean-Pierre Cartron, Carole Saison, Hein Hustinx, Thierry Peyrard, Bryan A. Ballif, Edmond Lee, Virginie Helias, Lucienne Mannessier, Shane Grimsley, Lionel Arnaud, and Geoff Daniels

Subjects

Nonsynonymous substitution, Male, Candidate gene, medicine.medical_specialty, Immunology, Nucleoside transporter, Equilibrative nucleoside transporter 1, Biochemistry, Polymorphism, Single Nucleotide, Protein Structure, Secondary, White People, Equilibrative Nucleoside Transporter 1, Ectopic calcification, Mice, medicine, Animals, Humans, Blood type, Mice, Knockout, biology, Transfusion Medicine, Ossification, Heterotopic, Cell Biology, Hematology, medicine.disease, Molecular biology, Null allele, Surgery, biology.protein, Blood Group Antigens, Female, Nucleoside

Abstract

The Augustine-negative alias At(a-) blood type, which seems to be restricted to people of African ancestry, was identified half a century ago but remains one of the last blood types with no known genetic basis. Here we report that a nonsynonymous single nucleotide polymorphism in SLC29A1 (rs45458701) is responsible for the At(a-) blood type. The resulting p.Glu391Lys variation in the last extracellular loop of the equilibrative nucleoside transporter 1 (ENT1; also called SLC29a1) is known not to alter its ability to transport nucleosides and nucleoside analog drugs. Furthermore, we identified 3 individuals of European ancestry who are homozygous for a null mutation in SLC29A1 (c.589+1GC) and thus have the Augustine-null blood type. These individuals lacking ENT1 exhibit periarticular and ectopic mineralization, which confirms an important role for ENT1/SLC29A1 in human bone homeostasis as recently suggested by the skeletal phenotype of aging Slc29a1(-/-) mice. Our results establish Augustine as a new blood group system and place SLC29A1 as a new candidate gene for idiopathic disorders characterized with ectopic calcification/mineralization.

Published

2015