Márcia Jorge Castejón

Blood collection on filter paper for HIV antibodies detection: experience of SampaCentro Project

Introduction: Blood samples collected on filter paper (dried blood spot [DBS]) is an immunoassay that has been used for antibodies screening. Objective: To evaluate the strategy of DBS blood collection for detection of HIV antibodies, evaluation of Q-Preven HIV 1 + 2 – DBS kit lot, and to analyze the stability of DBS samples. Method: Blood collection on DBS was performed according to World Health Organization (WHO) recommendations. The evaluation of the kit lot for HIV antibodies detection was performed using delta (d) values from the results of 774 DBS samples from volunteers men who have sex with men (MSM) recruited in the central region of Sao Paulo city, Brazil. Result: DBS blood collection was performed without complications. The positive (5.26) and negative (5.23) delta values allowed to clearly differentiate HIV antibodies reactive and non-reactive samples. We observed good performance of the kit lot and samples were stable on DBS form. Conclusion: Blood collection on DBS is feasible for the study of MSM population and is suitable for laboratory routine. The overall performance of Q Preven HIV-1 + 2 – DBS kit was satisfactory, having reached the quality levels required for the development of this study.

Estabilidade dos soros para o controle de qualidade interno de testes imunodiagnósticos de HIV/AIDS

Introduction: The use of reference materials in order to assure and perform the quality control of analytical measurements is a requirement in clinical laboratories. Objectives: Stability of serum samples, kept frozen at -20°C for long-term storage and at varied temperatures during short periods, was evaluated by investigating the persistency of anti-human immunodeficiency virus (HIV) antibodies reactivity on enzyme-linked immunosorbent assay/enzyme immunoassay (ELISA/EIA), Western blot and indirect immunofluorescence assays. Method: The analyzed sera were part of serum panels (comprised of anti-HIV positive and negative samples), produced at the Immunology Center of Instituto Adolfo Lutz, which have been the reference specimens for producing the internal quality assurance sera of HIV/acquired immunodeficiency syndrome (AIDS) immunodiagnostic assays. Sera stability was assessed in samples stored at -20°C for 56 weeks, and at various temperature conditions: from 2°C to 8°C (refrigerator), from 15°C to 25°C (room temperature), at 37°C (incubator) and at -80°C (freezer) for 24 and 48 hours. The statistical analyses on HIV-negative serum samples (long-term storage) were significant (p < 0.05), and neither adverse effects on these samples as the occurrence of false-positive results nor false-negative results in HIV antibody positive sera were found in both studies. Conclusion: It was possible to conclude that the reference material remained stable for 48 hours at different temperatures (short-term) and it remained stable at -20°C for 56 weeks (long-term).

Homogeneity study of the internal quality control sera for immunodiagnosis of HIV/AIDS

Introduction: The present study reports the data from the first homogeneity assessment of samples composing the serum panels produced at the Immunology Center of Instituto Adolfo Lutz, Sao Paulo. These samples have been distributed to the public laboratories and those partaking in the Brazilian Unified Health System, and to the participants in the Internal Quality Control Program for human immunodeficiency virus (HIV) antibody (Ab) testing. Objective: To assess the homogeneity of serum samples in panels from different lots for HIV/acquired immunodeficiency syndrome (AIDS) immunodiagnosis by using the statistical method to ensure quality of the reference material. Method: Sera homogeneity was evaluated by means of enzyme-linked immunoassay/enzyme immunoassay (ELISA/EIA) for detection of HIV Ab, and the one-way analysis of variance was employed for analyzing the data. No statistically significant differences were found among the several serum vials. Conclusion: The sera dispensed in the vials were homogeneous in the respective lots.

Study on the stability of HIV and syphilis reference materials under varied temperature conditions during their transportation

Introduction: The objective of this study was to evaluate the short-term stability of the serum samples used as internal quality control (IQC) of human immunodeficiency virus (HIV)/acquired immunodeficiency syndrome (Aids) and syphilis immunodiagnostic assays. These samples were produced at the Center of Immunology-Instituto Adolfo Lutz (IAL), and they were distributed to laboratories participating in the IAL Quality Control Program. Method: The sera analyzed by chemiluminescence assay were stored at varied temperature conditions: from 2oC to 8oC (refrigerator), from 15oC to 25oC (room temperature), at 37oC (incubator) and at -20oC (reference temperature) for 12 and 24 hours. Results: Comparative analysis of IQC results for anti-HIV and anti-T. pallidum (anti-treponemal) showed stability in the reference temperature and at the various simulated temperatures for transporting the samples at the established lengths of time. The data from the simple linear regression analysis of negative serum samples (incubator/24 hours) and in one batch of HIV IQC (room temperature/24 hours) were statistically significant at the level of 5% (p-value < 0.05). Conclusion: The sera presented necessary requirements as reference material to be transported to laboratories at refrigeration temperature (2oC to 8oC), at the maximum shipping time of 12 hours.

Performance validation of western blot for anti-HIV antibody detection in blood samples collected on filter paper (DBS)

Introduction: For conducting field studies on human immunodeficiency virus (HIV) serodiagnosis, the use of samples collected on filter paper [dried blood spot (DBS)] is profitable owing to the simplicity in handling and delivering them. Because of these characteristics, the use of DBS is recommended for studies in which the goal is to increase the population access to diagnostic testing, including HIV infection screening. For HIV diagnosis, the conventional strategy firstly uses an enzyme immunoassay as screening test, and the positive sample is confirmed on a complementary assay, as western blotting (WB). Objective: This study aimed at evaluating the analytical performance of WB assay for analyzing DSB samples. Method: One hundred eighteen blood samples collected in filter paper were analyzed by a modified WB. These samples derived from the SampaCentro Study, and they were HIV-antibody-positive in a screening test. In order to assess the reliability of these results, the assay performance was previously certified by employing the sample panel (reference panel) of Instituto Adolfo Lutz (IAL), which consisted of whole blood and plasma paired samples. Results: All of the DBS samples [100% (118/118)] showed the band pattern compatible with the criterion for HIV positivity established by the Ministry of Health. To validate the WB testing, the reciprocal relationship between antibody reactivity of DBS samples and of the respective plasma samples was investigated. Conclusion: WB optimization allowed the achievement of accurate results, and the easy DBS sample collection, transportation and storage will support the use of this immunodiagnostic technique for conducting HIV/acquired immunodeficiency syndrome (Aids) epidemiological surveys.

Efeito dos múltiplos ciclos de congelamento e descongelamento na estabilidade de amostras de soro antitreponêmico positivo

Introduction: Biological samples have long been used in multiple laboratory investigations, and this procedure has been an issue of concern, as the samples are submitted to repeated freeze-thaw cycles, which may affect the results of a particular immunodiagnostic assay, due to the occurrence of physical damage to the antibody of interest. Objective: This study aimed at investigating the impact of successive freeze-thaw cycles on the stability of serum samples stored at -20oC regarding the reactivity of anti-treponemal antibodies. Methods: At the Immunology Center-Instituto Adolfo Lutz (IAL), the analyzed serum samples analyzed were prepared and established as reference material for anti-treponemal immunodiagnostic assays. Sera stability was evaluated by chemiluminescence assay in samples submitted to 25 successive freeze-thaw cycles, ranging from 6 to 174 cycles. Results: Neither statistically significant effect on the reactivity of anti-treponemal antibodies (p-value > 0.05), nor adverse effect were observed in weakly reactive samples, such as the occurrence of false-negative results. Conclusion: It was shown that 174 freeze-thaw cycles of anti-treponemal sera did not affect the stability and the quality of samples, when evaluated by chemiluminescence assay.