ABSTRACT
Background: Paroxysmal nocturnal haemoglobinuria (PNH) clones in children are rare but commonly associated with aplastic anaemia (AA) and myelodysplasia.Objective: This study aimed to determine the prevalence of PNH clones in paediatric patients with idiopathic AA, identify differences in clinical and laboratory features and outcomes, and determine the impact of clone size on clinical presentation.Methods: Patients with confirmed idiopathic AA who were tested for PNH between September 2013 and January 2018 at the Inkosi Albert Luthuli Central Hospital, Durban, KwaZulu-Natal, South Africa, were included. PNH clones were detected in neutrophils and monocytes by flow cytometry using fluorescent aerolysin, CD24, CD66b and CD14. Results: Twenty-nine children with AA were identified and 11 were excluded. Ten patients (10/18, 55.6%) had PNH clones ranging from 0.11% to 24%. Compared to the PNH-negative group, these children were older (median: 10 years vs 4 years, p= 0.02) and had significantly lower total white cell counts (median 1.7 × 109/L vs 3.2 × 109/L; p= 0.04). There was no difference in median absolute neutrophil count or haemoglobin concentration. Four patients in each group received immunosuppressive therapy (IST). At six months, all four patients with PNH clones had responded, compared to one in the PNH-negative group. Conclusion: More than half of children with AA had a PNH clone. The size of the clone did not impact clinical severity; however, IST use may positively impact prognosis. We recommend early initiation of IST in patients with AA to avoid delays associated with human leukocyte antigen typing.
Subject(s)
Humans , Male , Female , Integrative Pediatrics , Anemia, Aplastic , Histocompatibility Testing , Dyspnea, Paroxysmal , Flow CytometryABSTRACT
Objective@#The Human Leukocyte Antigen (HLA) Class II is the major histocompatibility complex surface glycoproteins of humans responsible for presenting exogenous antigenic peptides which help direct specificity of immune response. In immune-cell therapy, the HLA allelic variants are of particular importance as they determine the successful activation of target cells that results to a desired therapeutic response. However, HLA Class II exhibits high polymorphism and has variable distribution in population, constituting these so-called allelic variants. Specifically, the HLA Class II DRB1 is considered the predominant locus among Filipinos. This research aimed to identify the presence of HLA Class II DRB1 allelic variants in the stem cell samples of ten (10) Filipino cancer patients by reverse transcription polymerase chain reaction (RT-PCR) amplification. @*Method@#This study employed a PCR-based HLA Class II typing to identify the HLA Class II DRB1 allelic variant in Filipino cancer patients. Design of forward and reverse primers for HLA Class II DRB1, optimization of PCR conditions for amplifying HLA Class II DRB1, and identification of HLA Class II DRB1 allelic variants from samples by sequencing and database comparison were conducted. @*Results@#PCR optimization showed that optimum annealing temperature for HLA DRB1 was 58.8°C with 1 mM MgCl2. PCR amplification of HLA DRB1 from ten anonymized cancer patient samples and DNA sequencing revealed that Patients 1, 2, 5, 8, 9, and 10 harbor HLA DRB1 allelic variants, particularly, the HLA DRB1*04:06:01, HLA DRB1*12:01:01, HLA DRB1*0813, HLA DRB1*04:05:01, HLA DRB1*09:01:02, and HLA DRB1*16:02:01, allelic variants, respectively.@*Conclusion@#Using the designed primers and optimized RT-PCR protocol, HLA information derived from six out of ten patient samples can be used for further applications in developing personalized or generic antigenic peptides such as dendritic cell cancer vaccine.
Subject(s)
HLA AntigensABSTRACT
BACKGROUND: Research on next-generation sequencing (NGS)-based HLA typing is active. To resolve the phase ambiguity and long turn-around-time of conventional high resolution HLA typing, this study developed a NGS-based high resolution HLA typing method that can handle large-scale samples within an efficient testing time. METHODS: For HLA NGS, the condition of nucleic acid extraction, library construction, PCR mechanism, and HLA typing with bioinformatics were developed. To confirm the accuracy of the NGS-based HLA typing method, the results of 192 samples HLA typed by SSOP and 28 samples typed by SBT compared to NGS-based HLA-A, -B and -DR typing. RESULTS: DNA library construction through two-step PCR, NGS sequencing with MiSeq (Illumina Inc., San Diego, USA), and the data analysis platform were established. NGS-based HLA typing results were compatible with known HLA types from 220 blood samples. CONCLUSION: The NSG-based HLA typing method could handle large volume samples with high-throughput. Therefore, it would be useful for HLA typing of bone marrow donation volunteers.
Subject(s)
Bone Marrow , Computational Biology , Gene Library , Histocompatibility Testing , HLA-A Antigens , Methods , Polymerase Chain Reaction , Statistics as Topic , VolunteersABSTRACT
Severe forms of dengue, such as dengue haemorrhagic fever (DHF) and dengue shock syndrome, are examples of a complex pathogenic mechanism in which the virus, environment and host immune response interact. The influence of the host's genetic predisposition to susceptibility or resistance to infectious diseases has been evidenced in several studies. The association of the human leukocyte antigen gene (HLA) class I alleles with DHF susceptibility or resistance has been reported in ethnically and geographically distinct populations. Due to these ethnic and viral strain differences, associations occur in each population, independently with a specific allele, which most likely explains the associations of several alleles with DHF. As the potential role of HLA alleles in the progression of DHF in Brazilian patients remains unknown, we then identified HLA-A alleles in 67 patients with dengue fever and 42 with DHF from Rio de Janeiro, Brazil, selected from 2002-2008 by the sequence-based typing technique. Statistical analysis revealed an association between the HLA-A*01 allele and DHF [odds ratio (OR) = 2.7, p = 0.01], while analysis of the HLA-A*31 allele (OR = 0.5, p = 0.11) suggested a potential protective role in DHF that should be further investigated. This study provides evidence that HLA class I alleles might be important risk factors for DHF in Brazilian patients.
Subject(s)
Adolescent , Adult , Aged , Aged, 80 and over , Child , Child, Preschool , Female , Humans , Male , Middle Aged , Young Adult , Severe Dengue/genetics , Genetic Predisposition to Disease/genetics , HLA-A1 Antigen/genetics , Alleles , Brazil , Case-Control Studies , Risk FactorsABSTRACT
En el ensayo de microlinfocitotoxicidad, el suero de conejo como fuente de complemento desempeña un rol esencial en la clasificación del complejo mayor de histocompatibilidad humano, tanto para la tipificación antigénica como en el cross-match linfocitario de la pareja donante-receptor antes de realizar los trasplantes. En este trabajo, se obtuvieron 3 lotes experimentales de dicho hemoderivado con óptimos indicadores de rendimiento, actividad biológica y estabilidad. El exanguíneo de los animales se realizó por la técnica de yugulación. El suero fue separado por centrifugación en condiciones ambientales y de temperatura controladas. Posteriormente, el producto se sometió a filtración esterilizante y se tomaron muestras para los ensayos de calidad. El estudio mostró que el producto conserva la actividad biológica al menos durante 18 meses y que los valores de citotoxicidad se encuentran dentro de los límites de aceptación para su empleo en los ensayos de histocompatibilidad pretrasplante
Microlinfocitotoxicity assay is one of the serological methods used to classify human major histocompatibility complex. In this technique the rabbit´s serum as complement source, plays an essential role in antigens determination and in lymphocytes cross match assay as necessary stage before the selection of the best donor-receiver pair to realize the organ transplant. Three experimental lots of normal rabbit serum were developed with excellent indicators of efficiency, biological activity and stability. Rabbit's blood was obtained through jugulating technique and serum was separated by centrifugation in controlled environment and temperature´s conditions. The sterilization process was performed by filtration and the samples were taken for quality´s control assays. Stability studies showed that the product kept the biological activity at least during 18 months after it was processed and cytotoxicity's values were adequate for its employment in histocompatibility pre-transplant assays
Subject(s)
Rabbits , Complement Hemolytic Activity Assay/methods , Histocompatibility Antigens , Organ Transplantation , Histocompatibility Testing/methodsABSTRACT
O Herpesvírus 8 humano (HHV-8) é endêmico em populações africanas e indígenas da região Amazônica. A infecção nestas populações acontece durante a infância e, na África, envolve o contato íntimo no ambiente intrafamiliar. Diversos estudos confirmam a distribuição geográfica dos diferentes subtipos de HHV-8, sendo que o subtipo E é típico das populações indígenas. Objetivos: 1. Caracterizar o(s) subtipo(s) de HHV-8 que circula(m) em população indígena da Amazônia brasileira baseado na análise da região ORF K1 do vírus; 2. Construir a árvore filogenética dos subtipos virais encontrados; 3. Comparar filogeneticamente os subtipos encontrados com os subtipos prevalentes em outras populações indígenas do Brasil e de outros países da América do Sul; 4. Calcular a taxa de substituição para a região VR1 do HHV-8 para as amostras estudadas; 5. Estimar a data de entrada do vírus na população do estudo; 6. Investigar a dinâmica de transmissão do vírus no ambiente intrafamiliar; 7. Averiguar se há correlação entre os alelos de HLA classe I (A e B) e II (DQB1 e DRB1) e suscetibilidade à infecção por HHV-8. Casuística e métodos: Estudo de soroprevalência da infecção por HHV-8 em amostra de população indígena da Amazônia brasileira utilizando IFI para detecção de antígenos da fase latente (LANA) e lítica (Lítico) do vírus. Análise filogenética da amostras encontradas utilizando-se o DNA/HHV-8 extraído de amostras de saliva, submetidas à reação de nested PCR para amplificar as regiões hipervariáveis VR1 e VR2. Cálculo da taxa de substituição do HHV-8, utilizando-se os métodos de distância e técnica bayesiana. Estimar a data do ancestral comum mais recente para as amostras em estudo, utilizando-se o programa BEAST. Tipagem de HLA de indivíduos positivos e negativos para a infecção por HHV-8, utilizando-se a técnica de PCR-SSO. Resultados: A soroprevalência geral da infecção por HHV-8 na população em estudo foi de 75,3% (399/530). Observou-se que a soropositividade...
The human herpesvirus 8 (HHV-8) is endemic in Africa and Amerindian populations from Amazon region. The infection in those populations occurs during childhood and, in Africa, involves a close contact in intrafamilial environment. Several studies confirm the geographical distribution of different subtypes of HHV-8, and the subtype E is typical of the Amerindian population. Objectives: 1. To characterize the HHV-8 subtypes circulating in Amerindian population from Brazilian Amazon, based on the analysis of ORF K1 region of the virus. 2. To construct a phylogenetic tree of viral subtypes found among Amerindians 3. To compare by phylogenetic methods the subtypes found in Mapuera Amerindians with the subtypes prevalent in others Amerindians populations of Brazil and South America 4. To determine the substitution rate of VR1 region of HHV-8 for the sequences obtained in the present study 5. To estimate the date of entry of the viruses in the Mapuera population 6. To investigate the dynamic of transmission of the virus in the intrafamilial environment 7. To investigate if there is a correlation between susceptibility to HHV-8-infection and HLA class I (A and B) and II (DQB1 and DRB1) alleles. Patients and methods: The seroprevalence of HHV-8 infection in a sample of the indigenous population of the Brazilian Amazon was carried out using IFA to detect antibodies to latent (LANA) and lytic phase antigens of HHV-8. Phylogenetic analysis of the sequences was performed by using the DNA extracted from samples of saliva, using a nested PCR to amplify the hypervariable regions VR1/ VR2 of HHV-8. Estimation of the substitution rate of HHV-8 nucleotides was performed by using the method of distance and the Bayesian technique. Estimates of the time of the most recent common ancestor (TMRCA) for all samples studied were done by using the BEAST program. HLA typing of positive and negative subjects for HHV-8 infection was performed by using the PCR-SSO technique...
Subject(s)
Humans , Male , Female , Biological Evolution , Histocompatibility Testing , Indigenous Peoples , Molecular Epidemiology , Seroepidemiologic StudiesABSTRACT
Oral submucous fibrosis (OSF) is now accepted globally as an Indian disease, having highest malignant potential than any other oral premalignant lesions. The understanding of the exact role of alkaloids and other etiological agents with respect to pathogenesis will help the management and minimize the blind clinical trials and treatment modalities. This article provides an overview of the etiopathogenesis with stress on the recent concepts related to this chronic “Indian Disease”.
Subject(s)
Oral Submucous Fibrosis , Arecoline , Oral Submucous Fibrosis , Histocompatibility TestingABSTRACT
BACKGROUND: To monitor the performance of histocompatibility testing laboratories, HLA proficiency survey in Korea has been conducted biannually since 1996. In this report, we summarized the results of the surveys performed in recent two years (2005-2006). METHODS: A total of four proficiency surveys were performed, in which 59-61 laboratories participated. Each survey included three tests for HLA class I (serology and DNA) and class II (DNA) typing and six tests for HLA crossmatch. RESULTS: The overall concordance of serologic typing was 98.9% (355/359) for HLA-A, 97.5% (350/ 359) for HLA-B, and 94.7% (337/356) for HLA-C. The antigens assigned correctly by less than 95% of the participating laboratories were A26 (93.8%), B38 (94.2%), Cw3/Cw10 (90.9%), Cw6 (94.4%), and Cw8 (74.3%). The overall concordance rates of DNA typing were 99.6% (533/535) for HLA-A, 99.8% (539/540) for HLA-B, and 100% (392/392) for HLA-C. Correct assignment of HLA-DRB1 and -DQB1 was reported by 99.2% (98.1-100%) and 96.7% (88.9-100%) for the generic level and 100% and 95.8% (75-100%) for the allelic level, respectively. On the average 3.8% (0-7.7%) of the total laboratories showed unacceptable results in the crossmatch tests. CONCLUSIONS: The rates of correct antigen identification and of unacceptable crossmatch were similar to those of previous surveys, which were considered satisfactory. The Korean proficiency survey program may have contributed to a high quality of HLA tests today and should be continued for further improvements of the tests tomorrow.
Subject(s)
Humans , Alleles , Data Collection , HLA Antigens/blood , HLA-A Antigens/blood , HLA-B Antigens/blood , HLA-C Antigens/blood , HLA-DQ Antigens/blood , HLA-DR Antigens/blood , Haplotypes , Histocompatibility Testing/standards , Korea , Laboratories , Quality ControlABSTRACT
BACKGROUND: HLA proficiency survey was started in 1996 in Korea, and the results of the 1996-1998 surveys were reported previously. Here, we report the results of the surveys performed in recent three years (2000-2002). METHODS: Six surveys were carried out with the participation of 52-54 laboratories. For each survey, 3 peripheral blood samples and 2 sera were distributed for 3 HLA class I serology, 3 HLA class I DNA, 3 HLA class II DNA, 6 HLA crossmatch, and 3 PRA tests. RESULTS: Overall consensus of serologic typing was similar to the results of the previous survey: HLA-A 93.5%, HLA-B 88.3%, and HLA-A, B 82.7%. There were an increasing number of the laboratories that were using DNA typing for HLA-DR (51 laboratories, 94%) and HLA-A and B (26 laboratories, 48%). Overall consensus of DNA typing was very high: HLA-A 100%, HLA-B 99.1%, HLAC 97.9%, HLA-DRB1 low/high resolution 99.2/99.0%, HLA-DQB1 low/high resolution 99.3/97.5%. HLA crossmatch (T cells) was reported by 44-49 laboratories, and the use of sensitive methods was increased: AHG 33 laboratories and flow cytometry 7 laboratories. For incompatible (positive) crossmatches, 4.9% (0-14.3%) of cytotoxicity tests and 7.1% (0-16.7%) of flow tests were reported as negative. PRA was reported by 5 laboratories only. CONCLUSIONS: The use of DNA tests for HLA typing and AHG or flow cytometry methods for HLA crossmatch tests has much increased compared to the previous report. A continuous survey program would play an important role in the standardization and maintenance of laboratory proficiency in histocompatibility testing in Korea.
Subject(s)
Consensus , DNA , DNA Fingerprinting , Flow Cytometry , Histocompatibility Testing , HLA-A Antigens , HLA-B Antigens , HLA-DR Antigens , HLA-DRB1 Chains , KoreaABSTRACT
BACKGROUND: HLA proficiency survey in Korea started in 1996 and the results of the survey were last reported in 1999. In this report, we summarized the results of the survey performed in recent 2 years. METHODS: A total of four proficiency surveys were performed, in which 54-59 laboratories participated. Each survey included 3 tests for HLA class I (serology and DNA) and class II (DNA) typing and 6 for HLA crossmatch test (3 cells x 2 sera). RESULTS: Overall concordance of serologic typing was 99.5% (436/438) for HLA-A, 95.7% (419/438) for HLA-B, and 94.8% (199/210) for HLA-C. The antigens assigned incorrectly by more than 5% of the participating laboratories were B54 (10.3%), B55 (10.3%), B27 (5.4%), Cw6 (22.9%), and C-blank (5.7%). Overall concordance rates of DNA typing were 99.7% (393/394) for HLA-A, 99.8% (415/416) for HLA-B, 100% (156/156) for HLA-C. Correct assignment of HLA-DRB1 and -DQB1 was reportred by 99.7% (98.1-100%) and 99.2% (88.9-100%) for generic and 99.2% and 98.1% (80-100%) for allelic level, respectively. Most laboratories (93.5-97.9%) were using sensitive methods of crossmatch such as T-long, T-AHG, and flowcytometry. The proportion of laboratories evaluated as unacceptable was on the average 3.1% of total laboratories. CONCLUSIONS: The rate of correct identification of HLA antigens was higher this time than in the previous survey in 1999. The rate of unacceptable crossmatch was also low enough to be satisfactory. It is thought that the proficiency survey has contributed to the high quality of HLA tests in the participating laboratories and should be continued to maintain the proficiency in Korea.
Subject(s)
DNA Fingerprinting , Histocompatibility Testing , HLA Antigens , HLA-A Antigens , HLA-B Antigens , HLA-C Antigens , HLA-DRB1 Chains , KoreaABSTRACT
BACKGROUND: The HLA system is known to be the most polymorphic gene cluster in the human genome. HLA allele and haplotype distribution varies widely among different ethnic groups. In this study, we examined the frequency of HLA class I alleles and haplotypes in 309 healthy Koreans. METHODS: We typed HLA-A, -B, and -C genes at the allelic level in 109 unrelated Korean individuals using a sequence-based typing. With the additional data of 200 healthy Koreans from dbMHC (http: //www.ncbi.nlm.nih.gov/mhc/), allele and haplotype frequencies were estimated by the maximum likelihood method. Serological typing results of 49 individuals were compared with the results highly resolved. RESULTS: A total of 22 HLA-A, 41 HLA-B, and 21 HLA-C alleles were found in this study. Alleles showing frequencies of more than 10% in each HLA locus were A*2402 (22.5%), A*0201 (15.7%), A*3303 (14.4%), A*1101 (11.0%), B*5101 (12.1%), Cw*0102 (18.8%), and Cw*1402 (10.2%). The most common A-B-C haplotypes at a frequency of more than 3% were A*3303-B*5801-Cw*0302 (5.2%), A*2402-B*5101-Cw*1402 (4.5%), A*1101-B*1501-Cw*0401 (4.3%), A*3303-B*4403-Cw*1403 (4.0%), A*3001-B*1302-Cw*0602 (3.7%), and A*0207-B*4601-Cw*0102 (3.2%). Misassignment of HLA-C antigen by serotyping was detected in 11 (22.4%) of 49 individuals. CONCLUSIONS: Our results will be useful as a basic data for studies on anthropology, disease association, and bone marrow transplantation. Misidentification of HLA-C by serotyping is so high that it would be desirable to perform a DNA typing especially in unrelated bone marrow transplantation.
Subject(s)
Humans , Alleles , Anthropology , Bone Marrow Transplantation , DNA Fingerprinting , Ethnicity , Genome, Human , Haplotypes , Histocompatibility Testing , HLA-A Antigens , HLA-B Antigens , HLA-C Antigens , Multigene Family , SerotypingABSTRACT
Objective:To study the relationship between human leukocyte antigen(HLA) typing, HLA crossreaction antigen group(CREGs) mismatching and early rejection after cadaver donor kidney transplantation.Methods:Donor and recipient HLA class Ⅰ typing was performed with Paul Terasaki monoclonal antibody tray and HLA class Ⅱ gene typing with Micro-sequence-specific-primers(Micro-SSP). PRA was detected by using Paul Terasaki mixture antigen tray.Results:The cases of 6, 5, 4, 3, 2, 1, 0 HLA mismatching(MM) in 131 recipients with negative PRA were respectively 0, 4, 26, 49, 33, 15, 4. The incidence of early rejection were 0,25%,23.1%,14.3%,12.1%,6.7%,0. No recipient with 5 and 6 CREGs MM. The case of 4,3,2,1,0 CREGs MM, the early rejection were respectively 28.6%,22.9%,9.5%,6.9%,5.5%.Conclusion:HLA typing and HLA crossreactive antigen group(CREGs) matching play an important role in selecting suitable donor, reducing early rejection, improving the effect of kidney transplantation.
ABSTRACT
There have been reports between Stevens-Johnson syndrome (SJS)induced by methazolamide treatment and genetic background especially in Japanese and Korean descent.We report 6 cases of SJS and the results of HLA (human leukocyte antigen)typing that suggest a relationship between genetic background and SJS induced by methazolamide treatment. We observed 6 patients as the subjects of this research, who had been suffering from SJS induced by methazolamide treatment at the Department of Ophthalmology, Catholic University.SJS appeared about 2 weeks after the patient started taking methazolamide (100 or 200 mg/d).After 15~30 days of treatment, they recovered with no serious complication.The results of HLA typing carried out 6 patients that all of the patients had HLA-A2, 5 patients were HLA-Cw1 and HLA-B59. Methazolamide should be carefully prescribed in patients of Japanese or Koreans descent and should not prescribe sulfonamide in SJS patients. A further systematic research on more cases is required to explaining ethnic peculiarity of the syndrome.
Subject(s)
Humans , Asian People , Histocompatibility Testing , HLA-A2 Antigen , Leukocytes , Methazolamide , Ophthalmology , Stevens-Johnson SyndromeABSTRACT
It is well known that HLA-B 27-associated uveitis is mostly anterior uveitis and has systemic manifestations.20 Patients [27 eyes]followed up at department of Ophthalmology of Kangnam St.Mary`s hospital, Catholic University Medical College from November 1989 to June 1998, were studied to delineate the clinical manifestations, treatments and prognosis in patients with HLA-B 27-associated uveitis.An HLA B27 associated systemic disorder was present in 10 patients, all of whom were ankylosing spondylitis. Systemic manifestations occurred in 19 patients included oral ulcer in 7 patients, genital ulcer in 3 patients, arthralgia in 16 patients, and skin lesion in 3 patients.Among the total 27 eyes, anterior uveitis was noted in 23 eyes and posterior segment involvement occurred in 4 eyes.The findings of posterior segment involvement included retinal vasulitis in 2 eyes and chorioretinitis in 1 eyes.Severe vitritis occurred in 1 eyes.Most of anterior uveitis was treated with topical steroid eyedrops and periocular steroid injections.In 3 eyes of posterior segment involvement, systemic steroid therapy was required for control of inflammation.After treatment, visual acuity in 23 eyes among 27 eyes was 20/40 or better.And, visual acuity in 4 eyes of posterior segment involvement was 20/25 or better following medical treatment.In conclusion, although HLA-B 27-associated uveitis was mostly related to anterior uveitis, posterior segment manifestations may be occurred in some patients;these patients may require the use of aggressive systemic immunosuppressive therapy to control inflammation and preserve vision.
Subject(s)
Humans , Arthralgia , Chorioretinitis , Histocompatibility Testing , HLA-B Antigens , Inflammation , Ophthalmic Solutions , Ophthalmology , Oral Ulcer , Prognosis , Retinaldehyde , Skin , Spondylitis, Ankylosing , Ulcer , Uveitis , Uveitis, Anterior , Visual AcuityABSTRACT
BACKGROUND: The most common problem in HLA typing is unsatisfactory quality of the antisera, or a lack of understanding of their reactivities. Therefore, commercial antisera must be verified under the conditions applied in a particular tissue typing laboratory. METHODS: We evaluated the antisera reactivities of a commercial HLA-yping tray, Lymphotype HLA-BC 72 oriental, the lot 7220999, 7230100 (Biotest, Germany), in about 300 samples from organ transplant recipients and healthy potential donors. RESULTS: The relatively weak antisera were those that defined A26, A33, Cw5, Cw14, B46, B58, B64 and B71 etc. Some of these antisera were not indicated as 'weak reaction' in the test result catalogue. The reactivities of each antisera indicated as 'extra reaction' or 'sometimes missing' were various. CONCLUSIONS: As for antisera reactivities, the data obtained by a laboratory itself are necessary in addition to those in the test result catalogue. These data will be helpful for the correct interpretation for laboratories using same commercial kits.
Subject(s)
Humans , Histocompatibility Testing , Immune Sera , Tissue Donors , TransplantsABSTRACT
BACKGROUND: The most common problem in HLA typing is unsatisfactory quality of the antisera, or a lack of understanding of their reactivities. Therefore, commercial antisera must be verified under the conditions applied in a particular tissue typing laboratory. METHODS: We evaluated the antisera reactivities of a commercial HLA-yping tray, Lymphotype HLA-BC 72 oriental, the lot 7220999, 7230100 (Biotest, Germany), in about 300 samples from organ transplant recipients and healthy potential donors. RESULTS: The relatively weak antisera were those that defined A26, A33, Cw5, Cw14, B46, B58, B64 and B71 etc. Some of these antisera were not indicated as 'weak reaction' in the test result catalogue. The reactivities of each antisera indicated as 'extra reaction' or 'sometimes missing' were various. CONCLUSIONS: As for antisera reactivities, the data obtained by a laboratory itself are necessary in addition to those in the test result catalogue. These data will be helpful for the correct interpretation for laboratories using same commercial kits.
Subject(s)
Humans , Histocompatibility Testing , Immune Sera , Tissue Donors , TransplantsABSTRACT
In order to evaluate association of particular HLA typing with certain uveitis in Korean population, HLA antigens were analyzed in 114 uneitis patients(acute anterior uveitis: 32 cases, Behcet`s disease: 25 cases, intermediate uveitis: 19 cases, Vogt-Koyanagi-Harada (V-K-H) syndrome: 10 cases, retinal vasculitis: 12 cases, Eale`s disease: 3 cases, posterior uveitis: 9 cases, pan.uveitis: 4 cases). The stronger association between acute anterior uveitis and HLA-B27 was statistically significant, and this result was similar to reports in other ethnic groups. Also, the association between V-K-H syndrome and HLA-DR4 showed same results. But the high frequency of HLA-DR7 in the patients with V-K-H syndrome was unque in patients of Korean popjlation and statistically significant. The association between HLA-A2 and posterior uveitis was high in patients of Korean population and statistically significant. Behcet`s disease was stronger association with HLA-B51 but not statistically significant and much weaker association than reports in Japanese group. Although many similarities of associations between particular uveitis and HLA typing were detected as compared with other ethnic groups, distinctive HLA associations were demonstrated in Korean population. Additional cases and long-term follow-up are required to confirm the association with HLA typing and the relationship with prognosis including clinical and laboratory variabilities.
Subject(s)
Humans , Asian People , Ethnicity , Follow-Up Studies , Histocompatibility Testing , HLA Antigens , HLA-A2 Antigen , HLA-B27 Antigen , HLA-B51 Antigen , HLA-DR4 Antigen , HLA-DR7 Antigen , Prognosis , Retinal Vasculitis , Uveitis , Uveitis, Anterior , Uveitis, Intermediate , Uveitis, PosteriorABSTRACT
BACKGROUND: We have performed questionnaire surveys of HLA laboratories in 1993 and 1995 and here we report the results of a survey performed in 1997. METHODS: The questionnaires were distributed to 39 HLA laboratories enrolled in the HLA quality assessment (QA) program (started in 1996) in Korea. The questionnaire items were slightly modified from those of the previous survey. RESULTS: Most of the HLA laboratories (31/39, 80%) belonged to the specialties of clinical pathology. Most of the HLA laboratories were of small scale in the number of HLA technicians and the annual number of HLA tests. The methods used for HLA crossmatch were quite improved compared to those of the previous survey (1995). The number of laboratories using sensitive methods such as T-AHG and/or T-long methods has markedly increased (31/34 laboratories, 91%) compared to that of the previous survey (5/29 laboratories, 17%). DNA typing methods for HLA-DR were used in 27 (69%) laboratories, among which 25 laboratories used commercial kits. Some laboratories stored complement at inappropriate temperature, which could adversely affect the test results. As for external QA programs for HLA tests, 7 laboratories were participating in international programs. Most of the laboratories responded that the domestic HLA QA program was of much help for HLA tests, especially for HLA crossmatch tests, and 21 laboratories changed the HLA crossmatch test methods after participating in the QA program. CONCLUSIONS: In recent 2 years, the most prominent changes in domestic HLA laboratories were increased use of HLA-DR DNA typing methods and improvement and standardization of HLA crossmatch test methods. The domestic HLA QA program was considered to be very helpful for quality improvement and standardization of HLA test.
Subject(s)
Complement System Proteins , DNA Fingerprinting , Histocompatibility Testing , HLA-DR Antigens , Korea , Pathology, Clinical , Quality Improvement , Surveys and QuestionnairesABSTRACT
Fifty-two Korean patients with Behcet's syndome were typed for HLA antigens. 52 apparently healthy Korean subjects were used as controls; 42 for HLA-A, B, C and all 52 for HLA-DR typing. HLA-B5 and DRw8 presented significantly high frequencies in all patiens. According to Shimizu's classification, HLA-B5 and DRw8 were significantly increased in the complete type; B5 in the incomplete type; DR3 in the suspected-possible type. According to Lehner's classification, HLA-DR3 was significantly increased in the neurological type; B5 in the ocular type; B5 in the ocular type. We confirmed the association of HLA-B5 with the severity of Beh et's syndrome. A relation might exist between DRw8, DR3 and Behcet's syndrome.