* Your assessment is very important for improving the workof artificial intelligence, which forms the content of this project
Download Overview of molecular methods in immunohematology
United Kingdom National DNA Database wikipedia , lookup
Site-specific recombinase technology wikipedia , lookup
Nutriepigenomics wikipedia , lookup
Point mutation wikipedia , lookup
Designer baby wikipedia , lookup
Non-coding DNA wikipedia , lookup
Nucleic acid double helix wikipedia , lookup
DNA supercoil wikipedia , lookup
Epigenomics wikipedia , lookup
Cre-Lox recombination wikipedia , lookup
Extrachromosomal DNA wikipedia , lookup
Molecular cloning wikipedia , lookup
Microevolution wikipedia , lookup
Therapeutic gene modulation wikipedia , lookup
Vectors in gene therapy wikipedia , lookup
Genealogical DNA test wikipedia , lookup
Deoxyribozyme wikipedia , lookup
DNA paternity testing wikipedia , lookup
History of genetic engineering wikipedia , lookup
Artificial gene synthesis wikipedia , lookup
Helitron (biology) wikipedia , lookup
Overview of molecular methods in immunohematology Marion E. Reid BACKGROUND B lood group antigens are inherited, polymorphic, structural characteristics located on proteins, glycoproteins, or glycolipids on the outside surface of the red blood cell (RBC) membrane. RBCs carrying a particular antigen can, if introduced into the circulation of an individual who lacks that antigen, elicit an immune response. It is the antibody from such an immune response that causes problems in transfusion incompatibility, maternal-fetal incompatibility, and autoimmune hemolytic anemia. The classical method of testing for blood group antigens and antibodies is hemagglutination. This technique is simple, inexpensive, and when carried out correctly, has a specificity and sensitivity that are appropriate for the clinical care of the vast majority of patients. However, hemagglutination, which is a subjective test, has certain limitations: 1) it does not reliably predict a fetus at risk of hemolytic disease of the newborn (HDN); 2) it is difficult to type RBCs from a patient who recently received a transfusion or those that are coated with IgG; 3) it does not precisely indicate RHD zygosity in D+ people; 4) a relatively small number of donors can be typed for a relatively small number of antigens, thereby limiting antigen-negative inventories; 5) it requires the availability of specific reliable antisera; 6) it is labor-intensive as is the manual data entry; 7) the source material is expensive and diminishing; 8) the cost of commercial reagents (Food and Drug Administration [FDA]-approved) is escalating; 9) many antibodies are not FDA-approved and are characterized (often partially) by the user; and 10) some antibodies are limited in volume, weakly reactive, or not ABBREVIATION: IRB = Institutional Review Board; SCD = sickle cell disease. From the Laboratory of Immunohematology, New York Blood Center, New York, New York. Address reprint requests to: Marion E. Reid, PhD, Laboratory of Immunohematology, New York Blood Center, 310 East 67th Street, New York, NY 10021; e-mail: mreid@ nybloodcenter.org. doi: 10.1111/j.1537-2995.2007.01304.x TRANSFUSION 2007;47:10S-16S. 10S TRANSFUSION Volume 47, July 2007 Supplement available. The understanding of the molecular bases associated with many blood group antigens and phenotypes enables us to consider the identification of blood group antigens and antibodies using molecular approaches. Screening donors by deoxyribonucleic acid (DNA) testing would conserve antibodies for confirmation by hemagglutination of predicted antigen negativity. The purpose of this overview was to discuss how molecular approaches can be used in transfusion medicine, especially in those areas where hemagglutination is of limited value. BLOOD TRANSFUSION SUPPORT IN PATIENTS WITH SICKLE CELL DISEASE (SCD) The Stroke Prevention Trial II corroborated the efficacy of continuous transfusions for preventing strokes in patients with SCD. So clear were the results that the National Heart, Lung, and Blood Institute aborted the 6-year trial after only 2 years. Of the proposed 100 patients, only 79 had been enrolled, 41 of whom were selected to discontinue transfusion. Of these, 14 reverted to high-risk transcranial Doppler ultrasound profiles and resumed transfusion. Of these 14 patients, 2 had suffered a stroke and received a transfusion, and 6 others resumed transfusion for other reasons.1 In contrast, none of the 38 patients who continued to receive transfusions had strokes or reverted to a high-risk state. The National Heart, Lung, and Blood Institute accordingly issued an alert to inform and advise physicians who treat children with SCD that interruption of transfusions for primary stroke prevention is not recommended. Unfortunately, one major risk of chronic transfusion therapy, whether given for stroke prevention or for other indications, is blood group alloimmunization with incidence rates of approximately 20 percent or higher, compared with 5 percent in other transfusion-dependent patient populations.2-6 Patients with SCD often produce many alloantibodies to blood group antigens, which makes the provision of appropriate antigen-negative blood very problematic. Our ability to test a large number of donors for minor antigens is restricted by laborintensive test procedures and data entry, and limited supplies or unavailability of typing grade antisera. Currently, patients with alloantibodies to multiple blood group MOLECULAR METHODS IN IMMUNOHEMATOLOGY PCR-based assays can be of value in the prenatal setting in identifying the fetus who is not at risk of HDN (i.e., predicted Antigen typing a patient • To identify a fetus at risk for HDN to be antigen-negative) so that the • When antibody is weak or not available, e.g., anti-Doa, -Dob, -Jsa, -V/VS mother need not be aggressively moni• Who has recently received a transfusion tored. Sources of fetal DNA include • Whose RBCs are coated with immunoglobulin (+DAT) • To distinguish an alloantibody from an autoantibody amniocytes and maternal plasma. • To detect weakly expressed antigens (e.g., Fyb with the FyX phenotype); where the DNA-based typing should be conpatient is unlikely to make antibodies to transfused antigen-positive RBCs sidered when a mother’s serum con• Identify molecular basis of unusual serologic results, especially Rh variants • To determine zygosity, particularly RHD tains an immunoglobulin G (IgG) Antigen typing for donors alloantibody that has been associated • To screen for antigen-negative donors with HDN and the father’s antigen • When antibody is weak or not available, e.g., anti-Doa, -Dob; -Jsa, -Jsb; -V/VS • Mass screening to increase antigen-negative inventory and to find donors whose RBCs status for the corresponding antigen is lack a high-prevalence antigen heterozygous, indeterminable, or he is • To resolve blood group A, B, D, C, and e discrepancies not available for testing. For prenatal • To detect genes that encode weak antigens • To type donors for reagent RBCs (antibody screening and identification panels) diagnosis of a fetus at risk of HDN, the Other applications approach to DNA typing should err on • One-step, automated, objective antibody detection and identification the side of caution. Thus, the strategy • Use of transfected cells as immunogens for production of monoclonal antibodies • Conversion of IgG monoclonal antibodies to IgM direct agglutinins should be to detect a gene even if the product is not expressed on the RBC membrane rather than fail to detect a antigens, or to an antigen of high prevalence, may have to gene whose product is expressed, because this could wait for matched RBC components to be obtained result in inadequate monitoring throughout pregnancy. through a national or even international Rare Donor RegAnother potential pitfall is the possibility of contaminaistry, or to undergo surgery with fewer units than the tion by maternal DNA. optimal. The unavailability of compatible blood may As the incidence of genes varies substantially in difextend hospital in-days (often in intensive care) and conferent populations, it can be helpful to know the ethnicity tributes to morbidity and mortality. If we are to transfuse of the parents. Also, to limit the gene pool, it is helpful to these patients effectively, we must find better ways of test DNA from the parents. An important practical considreducing the risk of transfusion reactions, hyperhemolysis eration is to determine whether the mother has undersyndrome, and alloimmunization. gone medical procedures such as artificial insemination, The genes encoding 28 of the 29 blood group systems in vitro fertilization, or whether she is a surrogate mother. (only the P system remains to be resolved) have been The RHD type is a prime target because anti-D is cloned and sequenced,7 and the molecular bases of blood notoriously clinically significant in terms of HDN group antigens and phenotypes have been determined.8 (reviewed in Avent and Reid10). DNA analysis for the preAnalysis of DNA involves amplification of the target diction of fetal D phenotype is based on detecting the sequence of nucleotides, followed by analysis by such presence or absence of portions of RHD. In Europeans, the techniques as polymerase chain reaction-restriction fragmolecular basis of the D– phenotype is usually associated ment length polymorphism (PCR-RFLP), allele-specific with deletion of the entire RHD, but several other molecuPCR, real-time PCR, sequencing, and microchip. The lar bases have been described.11 Approximately one-third results of DNA testing can be used to predict the presence of D– Japanese have an intact but inactive RHD,12 and as of blood group antigens in various scenarios, and to many as 10 percent of Japanese donors who had RBCs express antigens in heterologous systems not only to nonreactive with anti-D have the Del phenotype.13 detect and identify blood group antibodies in a single, Approximately one-quarter of D– African Americans have objective, automated assay but also as immunogens for an RHD pseudogene (RHDY), which does not encode the the production of monoclonal antibodies (Table 1).9 For D antigen,14 and many others have a hybrid RHD-CE-D the first time in the history of blood transfusion, microgene (e.g., the r’S phenotype). To predict the RhD antigen chip technology makes it feasible to contemplate precisely type by DNA analysis requires probing for multiple singlematching the antigen-negative status of a donor to that of nucleotide polymorphisms.15 Establishing the fetal K a patient destined to receive chronic transfusions. genotype is also of great clinical value in determining whether a fetus is at risk for severe anemia, because the DNA ASSAYS TO IDENTIFY A FETUS AT strength of the mother’s anti-K does not correlate with the RISK FOR ANEMIA OF THE NEONATE severity of the infant’s anemia.16 Hemagglutination, including titers, gives only an indirect When performing DNA analysis in the prenatal indication of HDN risk and severity. Antigen prediction by setting, it is also important to always determine the RHD TABLE 1. Clinical applications of molecular analyses Volume 47, July 2007 Supplement TRANSFUSION 11S REID status of the fetus, in addition to the test being ordered. In so doing, if the fetus has a normal RHD, there is no need to provide Rh- blood for interuterine transfusions. This is especially true if the mother has anti-c and fetal DNA is being typed for RHCE*c. DNA TYPING FOR BLOOD GROUP ANTIGENS FOR PATIENTS When a patient receives a transfusion, the presence of donor RBCs in the patient’s peripheral blood makes RBC phenotyping by conventional hemagglutination techniques complex, time-consuming, and possibly inaccurate. Indeed, the “best guess” of a patient’s antigen type based on the strength of hemagglutination, the number of RBC components transfused, the length of time since transfusion, the estimated blood volume of the patient, and the prevalence of the antigen in question is more often inaccurate than accurate.17 To overcome this problem, PCR-based assays using DNA isolated from white blood cells (WBCs), buccal smear, or urine sediment can be used to predict the antigen type of patients.18-21 DNA-based antigen typing of patients with autoimmune hemolytic anemia, whose RBCs are coated with immunoglobulin (have a positive direct antiglobutin test [DAT]), is valuable when 1) direct agglutinating antibodies, or murine monoclonal antibodies, are not available; 2) antisera are weakly reactive; 3) antigen is sensitive to the IgG removal treatment; and 4) diagnostic antibodies require the indirect antiglobulin test and IgG removal techniques are not effective at removing bound immunoglobulin. DNA-based assays are also useful as a tool to distinguish alloantibodies from autoantibodies and to identify the molecular basis of unusual serologic results. When recommendations for clinical practice are based on molecular analyses, it is important to remember that, in rare situations, a genotype determination will not correlate with antigen expression on the RBC.22 If a patient has a grossly normal gene that is not expressed, he or she could produce an antibody following transfusion of antigen-positive blood. When feasible, the appropriate assay to detect a mutation that silences a gene should be part of the DNA-based testing, e.g., GATA box and FY-265 analyses with FY typing,23 presence of RHD pseudogene with RHD typing,15 and exon 5 analysis with GYPBS typing.24 In addition, it is important to obtain an accurate medical history of the patient because with certain medical treatments, such as stem cell transplantation, results of DNA typing may differ from results obtained by hemagglutination. DNA TESTING FOR SCREENING BLOOD DONORS PCR-based assays can be used to predict the antigen type of the donor blood for transfusion and for antibody iden12S TRANSFUSION Volume 47, July 2007 Supplement tification reagent panels.25 This is particularly useful when antibodies are not available or are weakly reactive. Examples are Doa/Dob, Jsa, and V/VS where DNA-based assays are being used to type patients and donors to overcome the dearth of reliable typing reagents. PCRbased assays are also useful for confirming whether an antigen is truly present in a double dose, especially S, D, Fya, Fyb, Jka, and Jkb. In our laboratory, DNA-based assays were found to be valuable for differentiating specific Knops antigen negativity from a low copy number of CR1 (CD35). With donor typing, the presence of a grossly normal gene whose product is not expressed on the RBC surface would lead to the donor being falsely typed as antigenpositive, and although this would mean loss of an antigennegative donor, it would not jeopardize the safety of blood transfusion. As automated procedures attain higher and faster throughput at lower cost, typing of blood donors by DNA-based assays is likely to become more widespread. Screening for rare donors by analysis of DNA is valuable for typing for “minor” antigens and Rh variants. Those antigens that are predicted to be negative should be confirmed by hemagglutination. In this manner, precious antibodies are conserved for the confirmation of DNA typing predictions. Why not determine routine ABO and RHD by testing DNA? Like all donors, antigen-negative donors must have their ABO and Rh type determined. However, for several reasons DNA analysis is not the method of choice for routine ABO and D determination of donor blood. They include the following: the naturally occurring anti-A or anti-B in the plasma of most people who lack the corresponding antigens provides a built-in check when performing ABO typing by hemagglutination; potent, well-standardized monoclonal reagents are available for ABO and D typing; hemagglutination is relatively simple and rapid; and systems are in place to test and record, relatively efficiently, the ABO and D type of a donor. In both ABO and Rh systems, there are few antigens and many alleles. In the ABO system, there are four primary phenotypes (A, B, AB, O) but well over 100 alleles. In the Rh system, D is one antigen but there are close to 200 alleles known. In both scenarios, it is highly likely that more alleles exist and await detection. Furthermore, RBCs with a weak expression of the D antigen are almost always C+ or E+. Thus, the fear of transfusing apparently D– RBCs that actually express some serologically nondetectable D antigen can be more easily overcome by transfusing D– C– E– RBCs (which are usually truly D–) than by using DNA assays to detect the multiple alleles involved in the weak D phenotypes. For routine ABO and D determination, DNA testing is more time-consuming, more expensive, prone MOLECULAR METHODS IN IMMUNOHEMATOLOGY to misinterpretation, and not an improvement over hemagglutination. DNA analysis for ABO and Rh types can be of value in the resolution of ABO and D discrepancies, to show that a discrepancy is due to a genetic variant and not to technologist error or reagent failure and thus, not an FDA reportable error. ABO genotyping can also be useful for distinguishing an acquired phenotype from an inherited one without having to perform laborious family studies. Many Rh phenotypes cannot easily be defined by serologic methods, either because suitable panels of monoclonal antibodies are not readily available or because the antibodies are not available in the needed strength or volume. DNA assays may be useful for defining some and precisely match the D and e antigen status of a donor to a recipient, especially those with SCD. Testing for donors lacking Do antigens RBC typing for Doa, Dob, Hy, and Joa antigens of the Dombrock blood group system is notoriously difficult because the corresponding antibodies, although clinically significant, are often weakly reactive, available only in small volume, and present in sera containing other alloantibodies.26 At the New York Blood Center, PCR-RFLP analysis is used to type donors selected to lack certain combinations of antigens [e.g., C–, E–, K–, Fy(a–), Jk(b–)] for DOA and DOB for patients who have antibodies to such multiple antigens, in addition to anti-Doa or anti-Dob. Donors whose RBCs react weakly or do not react with human polyclonal anti-Gya for DO-HY and DO-JO are also tested. This has provided us with a larger inventory of valuable Hy– and Jo(a–) donors. Because of the dearth of appropriate antisera, testing for polymorphisms in the Dombrock system by DNA analysis surpasses hemagglutination for antigen typing. DNA typing for low-prevalence antigens Patients in New York often need Js(a–), V–, VS–, Go(a–), or DAK– RBC components. Providing RBC products for these patients is difficult because patients make antibodies to these antigens in addition to several others, e.g., anti-C, -E, -K, -Fya, and -Jkb. While these immunogenic antigens are of low prevalence in Caucasian donors, they are present on up to 20 percent of RBCs from African American donors. As a natural consequence of transfusing Rhand K-matched RBC components to patients, as in the Stroke Prevention Trials, the patients have made antibodies to these “low prevalence” antigens. These antigens are not on antibody screening RBCs; the corresponding antibodies are not available to screen for donors; and the crossmatch is not always reliable for their detection. PCRbased assays provide a tool to mass screen donors, thereby increasing the antigen-negative inventory and improving patient care. As an illustration, we had a patient whose serum contained anti-U, -C, -E, -K, plus -VS, and -Jsa. Of 95 eligible U– C– E– K– donors in the center’s inventory, four had been typed as VS–, Js(a–), 27 were VS+ or Js(a+), and 64 had not been typed for either antigen. Anti-VS and anti-Jsa were not available in sufficient volume for typing. PCR-based methods, which do not require special reagents, can be used to screen for antigen-negative donors. Current manual methods are time-consuming and labor intensive; however, the prospect of using microchips to screen large numbers of donors is appealing. This case is not unique, and many such examples throughout the United States exist. DNA typing for high-prevalence antigens As anti-Lub, -Yta, -Sc1, -LW, and -Coa are inconsistently available, testing DNA is a desirable alternative. The ready availability of anti-k, -Kpb, -Jsa, -Fy3, and -Jk3 often makes hemagglutination the method of choice for these antigens. On the other hand, if the appropriate singlenucleotide polymorphisms can be added to a microchip at little incremental cost, all of the above antigens could be predicted. Detection of Vel–, Lan–, At(a–), or Jr(a–) donors is restricted to hemagglutination because the molecular bases of these antigens are not yet known. Detection of null phenotypes such as Rhnull, K0, Gy(a–), Ge–, or McLeod is complex because of multiple molecular bases associated with these phenotypes.8 LIMITATIONS OF DNA ANALYSIS Testing by DNA analyses does have technical, medical, and genetic pitfalls.27 Medical pitfalls include recent transfusions, stem cell transplantation, and natural chimerism. In these scenarios, results of testing DNA may not agree with hemagglutination results. In addition, stem cell transplantation and natural chimerism may cause the results of testing DNA from somatic cells to differ from the results of testing DNA from WBCs. Thus, when embracing DNA testing, it is important to obtain an accurate medical history. There are many genetic events that cause apparent discrepant results between hemagglutination and DNA test results;28 the genotype is not the phenotype. The majority of DNA-based assays will detect a grossly normal gene that is not expressed and this can lead to a donor being falsely identified as antigenpositive. This would mean that a valuable antigennegative (e.g., null) donor would be lost to the inventory, but would not jeopardize the safety of a patient receiving blood transfusion. Confirmation by hemagglutination of predicted antigen negativity is recommended using a Volume 47, July 2007 Supplement TRANSFUSION 13S REID reagent antibody, if available, or by crossmatching using a method optimal for the detection of the antibody or antigen in question. Not all blood group polymorphisms can be easily analyzed, for example, if a large number of alleles encode one phenotype (e.g., ABO, Rh, and null phenotypes in many blood group systems); or alleles with a large deletion (e.g., Ge–) or alleles encoded by a hybrid gene (e.g., in the Rh and MNS systems); or when the molecular basis is not yet known (e.g., Vel, Lan, Jra). Additionally, there is a high probability that not all alleles in all ethnic populations are known. As discussed earlier, the molecular bases associated with a large number of antigens have been reported. However, in many cases, the analysis has been restricted to a relatively small number of people with known antigen profiles. This information is being applied to DNA typing with the assumption that such analysis will correlate with RBC antigen typing in all populations. However, we are still in our infancy of understanding gene polymorphisms in different ethnic groups and their significance to the expression of blood group antigens. A much larger number of people from a variety of ethnic backgrounds needs to be analyzed to establish more firmly the correlation between genotype and the blood group phenotype. Until such data are available, caution should be exercised when recommending clinical practice based on DNA typing for blood group antigens. MICROCHIP SCREENING FOR ANTIGEN-NEGATIVE DONORS Microchip technology simultaneously performs multiple assays on one sample; thereby a large number of antigens can be predicted on a large number of donor samples. The results are analyzed and interpreted by computer, and can be directly downloaded to a donor database, which will reduce data entry errors inherent in manual systems.29,30 The cost of the approach will depend on how much the manufacturers charge for kits they develop. An added cost of doing DNA testing could be the expense of investigating any discrepancies. High-throughput technologies have the potential to dramatically increase inventories of antigen-negative blood. POSSIBLE USES OF PHENOTYPICALLY MATCHED BLOOD If antigen-negative inventories were sufficient, the following uses of antigen-matched blood could be contemplated: • • • • TYPING BY DNA ASSAYS: CONCERN AND CONSENT Whether a study is considered exempt, expedited, or requires a full review by the Institutional Review Board (IRB) depends on several factors, namely, whether the samples are being tested for clinical purposes or research, whether the samples already exist or are collected specifically for the study, whether they are unlinked or linked, and whether there is a risk or not to the human subject. If a sample is tested for patient care, no IRB approval is needed. Donor consent may or may not be needed. This will depend on the wording of the local Donor Registration Form with regard to how the testing for blood groups antigens will be performed. There is much concern that testing DNA will reveal unwanted information about a donor. However, the assays are not considered “genotyping” but rather are a procedure to antigen type by DNA analysis. According to the New York State, as this DNA testing is not used to identify or diagnose a genetic disease, informed consent is not required. The interpretations do not differ from what can be presently accomplished by hemagglutination. 14S TRANSFUSION Volume 47, July 2007 Supplement • • • to match antigen profiles in chronically transfused patients who are immune responders, especially those with SCD disease; to match unusual Rh phenotypes, especially in African Americans (hrB–, hrS–, etc.); to predict the type of antigens for which there is no antibody (e.g., V/VS, Goa, DAK, Jsa, Doa, Dob); to match for Jka and Jkb if the patient has been exposed, to prevent transfusion reactions and deaths due to anti-Jka or anti-Jkb. Reports by the FDA in the United States and the Serious Hazards of Transfusion study in the UK have revealed that a handful of patients die annually after receiving transfusion of antigen-positive blood; to transfuse RBC components with weak expression of the RhD antigen to patients with similarly weak RhD expression (e.g., match for Del and Dweak); to transfuse patients with antibodies to high prevalence antigens; and to transfuse patients with autoimmune hemolytic anemia to eliminate labor-intensive procedures that are required to ensure that there are no underlying clinically significant antibodies. OTHER CONSIDERATIONS To apply molecular approaches to clinical situations, several areas of knowledge are needed, for example, a knowledge of molecular techniques, of gene structure and processing, of the molecular bases of blood groups, of hemagglutination techniques, of the expression of blood group antigens, of factors that may affect the interpretation of genotype (e.g., chimeras), and of regulatory com- MOLECULAR METHODS IN IMMUNOHEMATOLOGY pliance (Good Laboratory Practices, IRB, FDA), as well as an ability to correlate DNA and serologic results to the clinical problems being addressed. Numerous studies have analyzed blood samples from people with known antigen profiles and identified the molecular bases associated with many antigens. The available wealth of stockpiled serologically defined variants has contributed to the rapid rate with which the genetic diversity of blood group genes has been revealed. Initially, molecular information associated with each variant was obtained from only a small number of samples. This information was applied to DNA analyses with the hopeful assumption that the molecular analysis would correlate with RBC antigen typing. With the gathering of more information it became obvious that many molecular events result in the genotype and phenotype being apparently discrepant and that more than one genetic event can give rise to the same phenotype. This is especially true for null phenotypes, e.g., for Rh,8,31 Kell,26,32 and Kidd systems,32 and the p phenotype.33-34 Other considerations include establishing the extent of testing alleles for each antigen, e.g., GATA and nt FY-265 with FY typing, and whether to use the results without confirmation by hemagglutination if it is unlikely to harm the patient. If we had a simple, inexpensive way of positively identifying a donor at subsequent donations, DNA typing of a donor could be performed only once. Of value would be a system of automated DNA preparation and positive sample identification from the beginning of the process to the end. Hemagglutination is the gold standard technique to type RBCs for the presence or absence of blood group antigens. PCR-based assays, used as an adjunct to hemagglutination, will be a powerful tool that could radically change approaches used to support patients in their transfusion needs. 3. Heddle NM, Soutar RL, O’Hoski PL, et al. A prospective study to determine the frequency and clinical significance of alloimmunization post-transfusion. Br J Haematol 1995; 91:1000-5. 4. Redman M, Regan F, Contreras M. A prospective study of the incidence of red cell allo-immunisation following transfusion. Vox Sang 1996;71:216-20. 5. Aygun B, Padmanabhan S, Paley C, Chandrasekaran V. Clinical significance of RBC alloantibodies and autoantibodies in sickle cell patients who received transfusions. Transfusion 2002;42:37-43. 6. Rosse WF, Gallagher D, Kinney TR, et al. Cooperative study of sickle cell disease. Transfusion and alloimmunization in sickle cell disease. Blood 1990;76:1431-7. 7. Lögdberg L, Reid ME, Lamont RE, Zelinski T. Human blood group genes: chromosomal locations and cloning strategies. Transfus Med Rev 2005;19:45-57. 8. Reid ME, Lomas-Francis C. Blood group antigen factsbook, 2nd edition. San Diego, CA: Academic Press, 2004. 9. Yazdanbakhsh K. Applications of blood group antigen expression systems for antibody detection and identification. Transfusion 2007;47(Suppl):85S-8S. 10. Avent ND, Reid ME. The Rh blood group system: a review. Blood 2000;95:375-87. 11. Wagner FF, Frohmajer A, Flegel WA. RHD positive haplotypes in D negative Europeans. BMC Genet 2001;2:10. Available from http://www.biomedcentral.com/1471-2156/ 2/10. 12. Okuda H, Kawano M, Iwamoto S, et al. The RHD gene is highly detectable in RhD-negative Japanese donors. J Clin Invest 1997;100:373-9. 13. Chang JG, Wang JC, Yang TY, et al. Human RhDel is caused by a deletion of 1,013 bp between introns 8 and 9 including exon 9 of RHD gene. Blood 1998;92:2602-4. 14. Singleton BK, Green CA, Avent ND, et al. The presence of an RHD pseudogene containing a 37 base pair duplication ACKNOWLEDGMENT 15. Robert Ratner is acknowledged for his help in the preparation of the manuscript. 16. 17. REFERENCES 1. Adams RJ, Brambilla D. Optimizing Primary Stroke Prevention in Sickle Cell Anemia (STOP2) Trial Investigators. Discontinuing prophylactic transfusions used to prevent stroke in sickle cell disease. N Engl J Med 2005;353: 2769-78. 2. Hoeltge GA, Domen RE, Rybicki LA, Schaffer PA. Multiple red cell transfusions and alloimmunization: experience with 6996 antibodies detected in a total of 159,262 patients from 1985 to 1993. Arch Pathol Lab Med 1995;119:42-5. 18. 19. 20. and a nonsense mutation in Africans with the Rh D-negative blood group phenotype. Blood 2000;95:12-18. Westhoff C. Rh complexity. Serology and DNA genotyping. Transfusion 2007;47(Suppl):17S-22S. Lee S. The Kell and Kx blood group system. Transfusion 2007;47(Suppl):32S-9S. Reid ME, Oyen R, Storry J, Hue-Roye K, Rios M. Interpretation of RBC typing in multi-transfused patients can be unreliable. Transfusion 2000;40(Suppl):123S (Abstract). Wenk RE, Chiafari FA. DNA typing of recipient blood after massive transfusion. Transfusion 1997;37:1108-10. Legler TJ, Eber SW, Lakomek M, et al. Application of RHD and RHCE genotyping for correct blood group determination in chronically transfused patients. Transfusion 1999; 39:852-5. Reid ME, Rios M, Powell VI, Charles-Pierre D, Malavade V. DNA from blood samples can be used to genotype patients who have recently received a transfusion. Transfusion 2000;40:48-53. Volume 47, July 2007 Supplement TRANSFUSION 15S REID 21. Rozman P, Dovc T, Gassner C. Differentiation of autologous ABO, RHD, RHCE, KEL, JK, and FY blood group genotypes by analysis of peripheral blood samples of patients who have recently received multiple transfusions. Transfusion 2000;40:936-42. 22. Reid ME, Yazdanbakhsh K. Molecular insights into blood groups and implications for blood transfusions. Curr Opin Hematol 1998;5:93-102. 23. Castilho L. The value of DNA analysis for antigens in the Duffy blood group system. Transfusion 2007;47(Suppl): 28S-31S. antigen and antibody identification. Transfusion 2003;43: 1748-57. 29. Avent N. The BloodGen project: toward mass scale comprehensive genotyping of blood donors in the European Union and beyond. Transfusion 2007;47(Suppl):40S-46S. 30. Hashmi G. Red blood cell antigen phenotype by DNA analysis. Transfusion 2007;47(Suppl):60S-3S. 31. Huang C-H, Liu PZ, Cheng JG. Molecular biology and genetics of the Rh blood group system. Semin Hematol 2000;37:150-65. 24. Storry JR, Reid ME, Fetics S, Huang C-H. Mutations in GYPB exon 5 drive the S-s-U+var phenotype in persons of African descent: implications for transfusion. Transfusion 2003;43:1738-47. 32. Lee S, Russo DCW, Reiner AP, et al. Molecular defects underlying the Kell null phenotype. J Biol Chem 2001;276: 27281-9. 33. Lucien N, Sidoux-Walter F, Olivès B, et al. Characterization 25. Storry JR, Olsson M, Reid M. Application of DNA analysis to the quality assurance of reagent RBCs. Transfusion 2007; 47(Suppl):73S-8S. 26. Reid ME. Complexities of the Dombrock blood group system revealed. Transfusion 2005;45(Suppl):92S-9S. 27. Reid ME, Rios M. Applications of molecular genotyping to immunohaematology. Br J Biomed Sci 1999;56: 145-52. 16S TRANSFUSION 28. Reid ME. Applications of DNA-based assays in blood group Volume 47, July 2007 Supplement of the gene encoding the human Kidd blood group/urea transporter protein: evidence for splice site mutations in Jknull individuals. J Biol Chem 1998;273:12973-80. 34. Furukawa K, Iwamura K, Uchikawa M, et al. Molecular basis for the p phenotype. Identification of distinct and multiple mutations in the alpha 1,4-galactosyltransferase gene in Swedish and Japanese individuals. J Biol Chem 2000;275:37752-6.