Your search keyword '"laboratory proficiency testing"' showing total 1,310 results

1. Evaluating proficiency testing implementation and identifying challenges that government comprehensive specialized hospital laboratories in northwest Ethiopia faced as they participated in the external quality assessment scheme: A document-based, interview-driven evaluation

Author

Cherie, Negesse, Adane, Kasaw, Wolde, Maereg, Nigus, Mesele, and Deress, Teshiwal

Subjects

*MATERIALS testing, *PATHOLOGICAL laboratories, *CROSS-sectional method, *HOSPITALS, *PARTICIPATION

Abstract

Objectives To assess the implementation of proficiency testing in the northwest Ethiopian government comprehensive specialized hospital laboratories, with a focus on identifying and understanding the challenges encountered during their participation in the external quality assessment scheme. Methods A cross-sectional study was conducted among 3 comprehensive specialized hospitals in northwest Ethiopia, analyzing 41 documented laboratory test parameters from 2020 to 2022. In addition, face-to-face, in-depth interviews were carried out to identify the major challenges the participating institutions faced. Results The study covered a total of 41 tests across 9 cycles. Overall, proper implementation of proficiency testing was observed in 59.3% of the tests, with 61.8% maintaining consistent implementation status over 3 consecutive years. In addition, the overall performance of the laboratory was 54.3%, with a 68.7% participation rate. The predominantly identified challenges included the lack of participation, insufficient reagents and supplies, inadequacy of suitable proficiency testing materials, equipment malfunction and downtime, lack of management support, insufficient budget, and inadequate training and awareness. Conclusions The results of this study highlight the ineffective implementation of proficiency testing. Contributing factors include personnel issues, equipment and supplies challenges, managerial shortcomings, difficulties with proficiency testing providers, budgetary constraints, and a lack of training and motivation. [ABSTRACT FROM AUTHOR]

Published

2024

2. 我国精液分析外部质量评价中的问题及改进建议.

Author

李文娜, 徐晓倩, 石睛晴, 王民鑫, and 朱新兴

Abstract

External quality assessment (EQA) is the main way to evaluate whether the test results are accurate, and promote all laboratories to improve the testing quality. The EQA of semen analysis projects in China is still in its infancy and is only carried out in some areas. In the evaluation activities, there are some deficiencies, such as: (DEvaluation activities for the results of the permissible range is too large, which may be not conductive to discovering systematical errors in the laboratory. ②Allowing onsite assessment scores for personnel operations to replace laboratory evaluation; ®Tlie detection system in the evaluation activities adopt inconsistent with daily detection system •④The organizer pays insufficient attention on internal quality control of the participating; ®The application scope of EQA results is limited, etc ・ These deficiencies may result in the performance of the evaluation activities not truly reflecting to the laboratory testing capacity, which need further improvement. [ABSTRACT FROM AUTHOR]

Published

2024

3. Resultados del ejercicio de control de calidad externo 2022 de la Sociedad Latinoamericana de Genética Forense.

Author

Mireya Matamoros Zelaya, Joseph Alape Ariza, and Ixchel De la Luz Martínez

Subjects

forensic genetics, quality control, laboratory proficiency testing, Criminal law and procedure, K5000-5582, Medical legislation, K3601-3611, Public aspects of medicine, RA1-1270, Social pathology. Social and public welfare. Criminology, HV1-9960

Abstract

Introducción: La Sociedad Latinoamericana de Genética Forense, desde el año 2003 organiza ejercicios colaborativos de comparación interlaboratorios a fin de apoyar el fortalecimiento de los laboratorios de genética forense de Latinoamérica. Objetivo: presentar los resultados del análisis del ejercicio de calidad correspondiente al año 2022. Metodología: se diseñó un ejercicio práctico con cinco muestras: dos hisopados bucales (M1 y M2), una muestra de sangre en FTA (M3), una muestra mezcla de sangre-semen en FTA (M4) y un resto óseo (M5), siendo el ejercicio de calidad de SLAGF el único grupo que incluye en su ejercicio de calidad muestras óseas. Se envió además un ejercicio teórico con seis casos; dos contenían una mutación en un marcador especifico, uno consistió en una exclusión materna, otro de exclusión paterna, una paternidad sencilla trío y un caso de identificación de desaparecido, con muestras de referencia de presunta hija; su madre y abuela y tíos paternos, los ejercicios teóricos están disponibles en: http://slagf.org/resultados-control-slagf-2022/x Resultados: participaron 16 laboratorios y cinco peritos. En el ejercicio práctico, las muestras de mezcla y los restos óseos presentaron los mayores desafíos, el consenso por muestra fue de 100% para M1, de 93,75% para M2, de 87,5% para M3, 0% para M4 y de 75% para M5. El abordaje estadístico en los casos de identificación y la inclusión de mutaciones deben ser fortalecidos. Conclusión: los desafíos que enfrentan los laboratorios de genética forense latinoamericanos, reflejados por este ejercicio son similares a los encontrados por otros grupos que realizan ejercicios de calidad en Genética Forense.

Published

2022

4. Laboratorian Interpretation of Drug Testing Results in Pain Management: Lessons From College of American Pathologists Proficiency Testing.

Author

Snozek CLH, Langman LJ, Dizon A, and Krasowski MD

Subjects

Humans, United States, Pathologists, Drug Monitoring methods, Laboratories, Clinical, Pain Management methods, Laboratory Proficiency Testing

Abstract

Context.—: Accurate interpretation of drug test results is key to appropriate patient care in numerous settings, including pain management. Despite recommendations that providers should consult laboratory professionals for guidance when necessary, literature demonstrating laboratorian expertise in drug test interpretation is lacking., Objective.—: To evaluate participating laboratories' performance on the case-based, interpretive ("dry") challenge included with each Drug Monitoring for Pain Management proficiency testing program from 2012-2023., Design.—: All challenges (n = 23) required participants to identify if drug test results were consistent or inconsistent with prescribed medications in the case history. Relevant medications, presumptive and confirmatory drug test results, and participant responses were extracted from program summary reports and examined for performance and common themes., Results.—: Overall, 91.8% (6821 of 7431) of participant responses correctly identified whether drug testing was consistent with medications. There were 8 challenges with participant scores less than 91.8% (range, 59.8% [49 of 82 responses] to 88.9% [193 of 217 responses]). Common knowledge gaps identified in these challenges included false-positive presumptive (screening) results, minor metabolism of opiates, and recognizing that presence of a nonprescribed drug is inconsistent with prescribed medications. Although some participants repeatedly responded incorrectly, there were no associations between laboratory type, personnel responding, or analytical performance and incorrect responses to interpretative challenges., Conclusions.—: Program participants performed well overall, but several concerning educational gaps were identified. Laboratorians have a role in providing interpretative guidance for drug testing and should emphasize ongoing education to ensure competence in the setting of constantly changing prescribed and nonprescribed drug use., Competing Interests: The authors have no relevant financial interest in the products or companies described in this article., (© 2024 College of American Pathologists.)

Published

2024

5. Overview of proficiency testing results for the in vivo determination of sun protection factor.

Author

Zago DI, Ben Bari S, Tirard A, Miksa S, Renoux P, and Questel E

Subjects

Humans, Laboratory Proficiency Testing, Ultraviolet Rays, Sun Protection Factor, Sunscreening Agents

Abstract

A sunscreen product is allowed to be marketed if a protection is provided against ultraviolets (UV) including UVA rays and UVB rays expressed by the sun protection factor (SPF). UVB is radiation that is in the region of the ultraviolet spectrum which extends from about 290 to 320 nm in wavelength and that is primarily responsible for sunburn, ageing of the skin, and the development of skin cancer. Thus, since April 2009, the Bureau Interprofessionnel d'Etudes Analytiques (BIPEA) set up a proficiency testing scheme (PTS) for the determination of SPF in vivo of sunscreen products according to ISO 24444 standard [Cosmetics - Sun protection test methods - in vivo determination of the sun protection factor (SPF)] to evaluate the analytical performances of laboratories on these analyses. This PTS gathers twenty-six laboratories around the world with one trial a year. For each test, the statistical treatment of the data is performed according to ISO 13528 standard [Statistical methods for use in proficiency testing by interlaboratory comparison]. The assigned and tolerance values are calculated from the participants' data and the performances of the laboratories are evaluated individually and collectively according to ISO 17043 standard [Conformity assessment - General requirements for proficiency testing]. This paper presents the design of the PT program, its development, and an attentive analysis of laboratories results, which highlight the global performances obtained by laboratories on this type of analysis. The evaluation of the results shows, in fact, a relatively constant dispersion of data since the implementation of the PT program (variability between 10% and 50%)., (© 2024 Society of Cosmetic Scientists and Societe Francaise de Cosmetologie.)

Published

2024

6. International Proficiency Test Targeting a Large Panel of Botulinum Neurotoxin Sero- and Subtypes in Different Matrices.

Author

Rasetti-Escargueil C, Popoff MR, Kampa B, Worbs S, Marechal M, Guerin D, Paillares E, Luginbühl W, and Lemichez E

Subjects

Animals, Humans, Mass Spectrometry, Milk chemistry, Botulinum Toxins blood, Botulinum Toxins analysis, Botulinum Toxins immunology, Laboratory Proficiency Testing, Enzyme-Linked Immunosorbent Assay methods, Enzyme-Linked Immunosorbent Assay standards

Abstract

Detection of botulinum neurotoxins (BoNTs) involves a combination of technical challenges that call for the execution of inter-laboratory proficiency tests (PTs) to define the performance and ease of implementation of existing diagnostic methods regarding representative BoNT toxin-types spiked in clinical, food, or environmental matrices. In the framework of the EU project EuroBioTox, we organized an international proficiency test for the detection and quantification of the clinically relevant BoNT/A, B, E, and F sero- and subtypes including concentrations as low as 0.5 ng/mL. BoNTs were spiked in serum, milk, and soil matrices. Here, we evaluate the results of 18 laboratories participating in this PT. Participants have implemented a wide array of detection methods based on functional, immunological, and mass spectrometric principles. Methods implemented in this proficiency test notably included endopeptidase assays either coupled to mass spectrometry (Endopep-MS) or enzyme-linked immunosorbent assays (Endopep-ELISA). This interlaboratory exercise pinpoints the most effective and complementary methods shared by the greatest number of participants, also highlighting the importance of combining the training of selected methods and of distributing toxin reference material to reduce the variability of quantitative data.

Published

2024

7. An interlaboratory proficiency test using metagenomic sequencing as a diagnostic tool for the detection of RNA viruses in swine fecal material.

Author

Liu L, Hakhverdyan M, Wallgren P, Vanneste K, Fu Q, Lucas P, Blanchard Y, de Graaf M, Oude Munnink BB, van Boheemen S, Bossers A, Hulst M, and Van Borm S

Subjects

Animals, Swine, Computational Biology methods, Genome, Viral genetics, Laboratory Proficiency Testing, RNA, Viral genetics, Astroviridae Infections veterinary, Astroviridae Infections diagnosis, Astroviridae Infections virology, Metagenome, High-Throughput Nucleotide Sequencing methods, Feces virology, Metagenomics methods, Swine Diseases virology, Swine Diseases diagnosis, RNA Viruses genetics, RNA Viruses isolation & purification, RNA Viruses classification

Abstract

Metagenomic shotgun sequencing (mNGS) can serve as a generic molecular diagnostic tool. An mNGS proficiency test (PT) was performed in six European veterinary and public health laboratories to detect porcine astroviruses in fecal material and the extracted RNA. While different mNGS workflows for the generation of mNGS data were used in the different laboratories, the bioinformatic analysis was standardized using a metagenomic read classifier as well as read mapping to selected astroviral reference genomes to assess the semiquantitative representation of astrovirus species mixtures. All participants successfully identified and classified most of the viral reads to the two dominant species. The normalized read counts obtained by aligning reads to astrovirus reference genomes by Bowtie2 were in line with Kraken read classification counts. Moreover, participants performed well in terms of repeatability when the fecal sample was tested in duplicate. However, the normalized read counts per detected astrovirus species differed substantially between participants, which was related to the different laboratory methods used for data generation. Further modeling of the mNGS data indicated the importance of selecting appropriate reference data for mNGS read classification. As virus- or sample-specific biases may apply, caution is needed when extrapolating this swine feces-based PT for the detection of other RNA viruses or using different sample types. The suitability of experimental design to a given pathogen/sample matrix combination, quality assurance, interpretation, and follow-up investigation remain critical factors for the diagnostic interpretation of mNGS results., Importance: Metagenomic shotgun sequencing (mNGS) is a generic molecular diagnostic method, involving laboratory preparation of samples, sequencing, bioinformatic analysis of millions of short sequences, and interpretation of the results. In this paper, we investigated the performance of mNGS on the detection of porcine astroviruses, a model for RNA viruses in a pig fecal material, among six European veterinary and public health laboratories. We showed that different methods for data generation affect mNGS performance among participants and that the selection of reference genomes is crucial for read classification. Follow-up investigation remains a critical factor for the diagnostic interpretation of mNGS results. The paper contributes to potential improvements of mNGS as a diagnostic tool in clinical settings., Competing Interests: The authors declare no conflict of interest.

Published

2024

8. Identification methods as a factor affecting the performance of clinical microbiology laboratories participating in an external quality assessment program: a cross-sectional, retrospective analysis.

Author

Wu J, Alam MS, Restelli V, Vimalanathan S, and Perrone LA

Subjects

Cross-Sectional Studies, Humans, Retrospective Studies, Canada, Bacteria isolation & purification, Bacteria classification, Quality Assurance, Health Care, Bacteriological Techniques standards, Bacteriological Techniques methods, Quality Control, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization standards, Laboratory Proficiency Testing, Laboratories, Clinical standards

Abstract

Introduction. Laboratory participation in external quality assessment (EQA) programmes including proficiency testing (PT) is a requirement of clinical laboratory conformance to ISO 15189:2022 Medical laboratories - Requirements for quality and competence . PT is one EQA method whereby laboratories are sent blinded samples for characterization by routine laboratory diagnostic methods. Importantly, PT enables a laboratory's performance to be evaluated in comparison to the standard reference methods and to the performance of other peer laboratories using similar diagnostic methods. Gap statement. The desired outcome of participating in PT is to help laboratories identify possible sources of error in each step of the total testing process and particularly in their test methods during the analytical phase. Aim. This cross-sectional study investigated the impact of using matrix-assisted laser desorption ionization time-of-flight mass spectrometry (MALDI-TOF MS) compared to conventional phenotypic biochemical testing on laboratory performance in a clinical bacteriology PT scheme. Methodology. During a 6-year period from 2017-2022, the Canadian Microbiology Proficiency Testing implemented 112 PT challenges comprising 22 different sample types and included 61 different bacterial species. This was translated into 5883 graded test events for analysis. Multiple logistic regression techniques were employed to explore the association between the test method employed and laboratory performance. The sample type and aerobic classification of challenge organisms were included as confounding variables. Results. Laboratories using MALDI-TOF MS performed significantly better in characterizing microorganisms than laboratories using phenotypic biochemical testing alone [odds ratio OR = 5.68, confidence interval (CI): 3.92, 8.22] regardless of the sample type and aerobic classification. Notably, our analysis identified a significant association between anaerobic organisms and laboratory performance (OR: 0.24, CI: 0.17-0.35), suggesting that culturing and identifying fastidious organisms remains a significant obstacle for many clinical microbiology laboratories. Conclusions. Although no method is infallible and its performance will depend on the validation and quality assurance procedures, this finding may help the management in the decision for implementing MALDI-TOF MS in the microbiology laboratory. This study highlights the important role PT providers play in the objective assessment of laboratory performance and how it can provide evidence for quality improvement.

Published

2024

9. Continuous Global Improvement of Human Papillomavirus (HPV) Genotyping Services: The 2022 and 2023 HPV LabNet International Proficiency Studies.

Author

Arroyo Mühr LS, Eklund C, Lagheden C, Yilmaz E, Forslund O, Lilja M, and Dillner J

Subjects

Humans, Global Health, Sensitivity and Specificity, Human Papillomavirus Viruses, Papillomavirus Infections virology, Papillomavirus Infections diagnosis, Genotyping Techniques methods, Genotyping Techniques standards, Papillomaviridae genetics, Papillomaviridae classification, Papillomaviridae isolation & purification, Genotype, Laboratory Proficiency Testing

Abstract

The International Human Papillomavirus (HPV) Reference Center launches annual global HPV genotyping proficiency panels to enhance the precision and international standardization of HPV genotyping services. This study aims to assess the proficiency levels achieved in the global HPV genotyping proficiency panels conducted in 2022 and 2023, and to evaluate trends in performance over time. The proficiency panels comprised 44 blinded samples each, including 40 samples containing various purified plasmids corresponding to HPV types combined with human DNA, plus four control samples (one negative control and three extraction controls). Proficiency required a sensitivity of 50 International Units (IU)/5 µL for HPV 16 and HPV 18 500 IU/5 µL for HPVs 6, 11, 31, 33, 45, 52, and 58 and 500 genome equivalents (GE)/5 µL for other HPV types in both single and multiple infections, while avoiding false positivity. In 2022, 78 laboratories submitted a total of 154 data sets, and in 2023, 81 laboratories contributed 141 data sets. Most data sets (87%, 258/295) utilized commercially available HPV assays. Proficiency was common, with 77% of data sets meeting the proficiency criteria in 2022 and 79% in 2023. False positive results significantly decreased from 22% in 2022 to 13% in 2023. The high proficiency and increasing specificity in HPV genotyping services indicates progress toward more reliable HPV testing. High accuracy is crucial for supporting global efforts in HPV and cervical cancer elimination., (© 2024 The Author(s). Journal of Medical Virology published by Wiley Periodicals LLC.)

Published

2024

10. Harmonizing lipidomics: NIST interlaboratory comparison exercise for lipidomics using SRM 1950-Metabolites in Frozen Human Plasma.

Author

Bowden, John, Heckert, Alan, Ulmer, Candice, Jones, Christina, Koelmel, Jeremy, Abdullah, Laila, Ahonen, Linda, Alnouti, Yazen, Armando, Aaron, Asara, John, Bamba, Takeshi, Barr, John, Bergquist, Jonas, Borchers, Christoph, Brandsma, Joost, Breitkopf, Susanne, Cajka, Tomas, Cazenave-Gassiot, Amaury, Checa, Antonio, Cinel, Michelle, Colas, Romain, Cremers, Serge, Gardner, Michael, Garrett, Timothy, Gotlinger, Katherine, Han, Jun, Huang, Yingying, Neo, Aveline, Hyötyläinen, Tuulia, Izumi, Yoshihiro, Jiang, Hongfeng, Jiang, Houli, Jiang, Jiang, Kachman, Maureen, Kiyonami, Reiko, Klavins, Kristaps, Klose, Christian, Köfeler, Harald, Kolmert, Johan, Koal, Therese, Koster, Grielof, Kuklenyik, Zsuzsanna, Kurland, Irwin, Leadley, Michael, Lin, Karen, Maddipati, Krishna, McDougall, Danielle, Meikle, Peter, Mellett, Natalie, Monnin, Cian, Moseley, M, Nandakumar, Renu, Oresic, Matej, Patterson, Rainey, Peake, David, Pierce, Jason, Post, Martin, Postle, Anthony, Pugh, Rebecca, Qiu, Yunping, Ramrup, Parsram, Rees, Jon, Rembiesa, Barbara, Reynaud, Denis, Roth, Mary, Sales, Susanne, Schuhmann, Kai, Schwartzman, Michal, Serhan, Charles, Shevchenko, Andrej, Somerville, Stephen, St John-Williams, Lisa, Surma, Michal, Takeda, Hiroaki, Thakare, Rhishikesh, Thompson, J, Torta, Federico, Triebl, Alexander, Trötzmüller, Martin, Ubhayasekera, S, Vuckovic, Dajana, Weir, Jacquelyn, Welti, Ruth, Wenk, Markus, Wheelock, Craig, Yao, Libin, Yuan, Min, Zhao, Xueqing, Zhou, Senlin, Evans, James, Fauland, Alexander, Dennis, Edward, Fiehn, Oliver, and Quehenberger, Oswald

Subjects

National Institute of Standards and Technology, Standard Reference Material 1950, fatty acyls, glycerolipids, lipids, phospholipids, quality control, quantitation, sphingolipids, sterols, Benchmarking, Humans, International Cooperation, Laboratory Proficiency Testing, Lipid Metabolism, Lipids, Observer Variation, Reference Standards, Reproducibility of Results

Abstract

As the lipidomics field continues to advance, self-evaluation within the community is critical. Here, we performed an interlaboratory comparison exercise for lipidomics using Standard Reference Material (SRM) 1950-Metabolites in Frozen Human Plasma, a commercially available reference material. The interlaboratory study comprised 31 diverse laboratories, with each laboratory using a different lipidomics workflow. A total of 1,527 unique lipids were measured across all laboratories and consensus location estimates and associated uncertainties were determined for 339 of these lipids measured at the sum composition level by five or more participating laboratories. These evaluated lipids detected in SRM 1950 serve as community-wide benchmarks for intra- and interlaboratory quality control and method validation. These analyses were performed using nonstandardized laboratory-independent workflows. The consensus locations were also compared with a previous examination of SRM 1950 by the LIPID MAPS consortium. While the central theme of the interlaboratory study was to provide values to help harmonize lipids, lipid mediators, and precursor measurements across the community, it was also initiated to stimulate a discussion regarding areas in need of improvement.

Published

2017

11. Trends in Cervical Cytology Screening and Reporting Practices: Results From the College of American Pathologists 2011 PAP Education Supplemental Questionnaire

Author

Crothers, Barbara A, Darragh, Teresa M, Tambouret, Rosemary H, Nayar, Ritu, Barkan, Guliz A, Zhao, Chengquan, Booth, Christine Noga, Padmanabhan, Vijayalakshmi, Tabatabai, Z Laura, Souers, Rhona J, Thomas, Nicole, Wilbur, David C, and Moriarty, Ann T

Subjects

Reproductive Medicine, Biomedical and Clinical Sciences, Prevention, Cross-Sectional Studies, Early Detection of Cancer, Female, Gynecology, Humans, Image Interpretation, Computer-Assisted, Laboratories, Laboratory Proficiency Testing, Pathology, Clinical, Quality Assurance, Health Care, Surveys and Questionnaires, United States, Uterine Cervical Neoplasms, Vaginal Smears, Workload, Clinical Sciences, Pathology, Clinical sciences

Abstract

ContextThe College of American Pathologists periodically surveys laboratories to determine changes in cytopathology practices. We report the results of a 2011 gynecologic cytology survey.ObjectiveTo provide a cross-sectional survey of gynecologic cytology practices in 2010.DesignIn 2011, a survey was sent to 1604 laboratories participating in the College of American Pathologists gynecologic cytology interlaboratory comparison education program and proficiency testing programs requesting data from 2010 on the following topics: terminology/reporting, cytotechnologist workload, quality assurance, reagents, and ancillary testing.ResultsSix hundred and twenty-five laboratories (39%) replied to the survey. The nonstandard use of "low-grade squamous intraepithelial lesion cannot exclude high-grade squamous intraepithelial lesion" is used by most laboratories to report the presence of low-grade squamous intraepithelial lesion with possibility of high-grade squamous intraepithelial lesion. Most laboratories also report the presence or absence of cells from the transformation zone. Most respondents do not limit cytotechnologist screening workload during the work shift. Only about one-third of laboratories (188 of 582; 32%) use image-assisted screening devices. Rapid prescreening as a quality assurance measure is used by only 3.5% (21 of 594) of the laboratories. When used for screening, most laboratories use the imager for retrospective review of slides to detect human locator and interpretive errors. Most laboratories receive both liquid-based cytology samples (mainly ThinPrep, Hologic, Marlborough, Massachusetts) and conventional Papanicolaou tests. Expiration dates of liquid-based cytology test vials are not usually recorded.ConclusionsThe field of gynecologic cytology is evolving rapidly. These survey results offer a snapshot of national gynecologic cytology practices in 2010.

Published

2016

12. Reproducibility of Fluorescent Expression from Engineered Biological Constructs in E. coli.

Author

Beal, Jacob, Haddock-Angelli, Traci, Gershater, Markus, de Mora, Kim, Lizarazo, Meagan, Hollenhorst, Jim, Rettberg, Randy, and iGEM Interlab Study Contributors

Subjects

iGEM Interlab Study Contributors, Escherichia coli, Green Fluorescent Proteins, Reproducibility of Results, Protein Engineering, Transcription, Genetic, Promoter Regions, Genetic, Transcriptional Activation, Laboratory Proficiency Testing, General Science & Technology

Abstract

We present results of the first large-scale interlaboratory study carried out in synthetic biology, as part of the 2014 and 2015 International Genetically Engineered Machine (iGEM) competitions. Participants at 88 institutions around the world measured fluorescence from three engineered constitutive constructs in E. coli. Few participants were able to measure absolute fluorescence, so data was analyzed in terms of ratios. Precision was strongly related to fluorescent strength, ranging from 1.54-fold standard deviation for the ratio between strong promoters to 5.75-fold for the ratio between the strongest and weakest promoter, and while host strain did not affect expression ratios, choice of instrument did. This result shows that high quantitative precision and reproducibility of results is possible, while at the same time indicating areas needing improved laboratory practices.

Published

2016

13. External quality assessment program for biochemical assays of human seminal plasma: a French 6-years experience

Author

Safouane M. Hamdi, Erick Sanchez, Delphine Garimbay, and Stéphanie Albarede

Subjects

Laboratory proficiency testing, ISO 15189, Seminal plasma, Biomarkers, Male genitalia, Citrate, Medicine (General), R5-920

Abstract

Résumé CONTEXTE Malgré un usage ancien, ce n’est qu’en 1999 que l’OMS propose dans son manuel d’examen du sperme humain de doser plusieurs composés biochimiques du plasma séminal pour l’exploration fonctionnelles des glandes annexes. A la même période, un effort international s’organise pour standardiser les examens de laboratoires et augmenter leur performance avec l’accréditation selon la norme ISO 15189. Dans ce contexte, la participation des laboratoires aux programmes d’évaluation externe de la qualité (EEQ) est une exigence fondamentale. Afin de les aider à faire face à cette obligation, nous avons organisé un EEQ pour la biochimie séminale basé sur des échantillons commutables. Dans ce travail, nous souhaitons rapporter une vue globale sur l’offre analytique française, sur les méthodes de dosage utilisées et leurs performances. Nous évaluons également leur potentiel à répondre aux exigences de la norme concernant l’accréditation. RESULTATS Nous avons proposé entre 2014 et 2019 sept enquêtes. Une médiane de six laboratoires a répondu à chaque enquête, soit un ratio d’un laboratoire pour 11.2 millions d’habitants. Sept marqueurs séminaux sont dosés en routine mais un noyau dur de 4 marqueurs est partagé par tous les laboratoires: citrate, zinc (prostate), fructose (vésicules séminales) et α-1,4 glucosidase (épididyme). L’usage de méthodes marquées CE-IVD a concerné entre 0 et 75% de l’ensemble des dosages. Tous les laboratoires ont rendu des résultats de zinc dans les limites acceptables définies, 75% pour le citrate et α-1,4 glucosidase et 67% pour le fructose. En combinant toutes les données recueillies, nous avons construit un score qui a permis de classer le potentiel d’accréditation des marqueurs séminaux: l’accréditation du citrate, fructose et zinc ne devrait pas poser problème, l’ α-1,4 glucosidase présente une faiblesse analytique mais la phosphatase prostatique, la L-carnitine libre et la glycérophosphocholine ne sont pas accréditables en l’état actuel. Conclusion Nous avons organisé un programme d’EEQ de biochimie séminale pour aider les laboratoires français à répondre à l’exigence d’accréditation totale en 2020. Ce programme est. perfectible mais il a permis de révéler les forces et faiblesses de ce paysage analytique. Des méthodes sont disponibles pour une exploration biochimique efficiente de la prostate et des vésicules séminales mais celle des épididymes est apparue particulièrement fragile. Ce problème andrologique doit être pris en compte par les autorités sanitaires et les sociétés savantes concernées.

Published

2020

14. Sigma Metrics-Tool for Quality Assurance in Clinical Biochemistry Laboratory

Author

Richa Singh and MN Vanitha Gowda

Subjects

bias, laboratory proficiency testing, quality control, quality goal index, Microbiology, QR1-502, Chemistry, QD1-999

Abstract

Introduction: Sigma metrics is a quality management tool used for process improvement which usually comes into application when there is a measurable outcome in the process. It can play an important role in health care laboratory services as Quality Assurance (QA) of the same, is the need of the hour. Aim: To gauge the performance of a few biochemical parameters by calculating their sigma metrics on a sigma scale. Materials and Methods: This retrospective study was undertaken using Quality Control (QC) and External QA Scheme (EQAS) data for 17 biochemical parameters from Biochemistry section, diagnostic laboratory of an M.S. Ramaiah Medical College and Hospital, Bengaluru. Sigma values for these parameters were determined and sigma metrics was evaluated for duration of 13 months. Results: In level 1 coefficient of variation percentage (CV%), five parameters (ALP, calcium, magnesium, triglycerides and HDL-cholesterol) showed an ideal performance of ≥6 sigma level and in level 2 CV%, eight parameters (total bilirubin, urea, creatinine, albumin, AST, total cholesterol, total protein and phosphorus) showed a sigma of ≥6. Quality Goal Index (QGI) for 11 analytes in level 1 and seven analytes in level 2 was

Published

2020

15. Proficiency testing for event-specific quantification of genetically modified maize MON87427: Performance assessment based on the metrologically traceable reference values as assigned values.

Author

Wang D, Fei Y, Niu C, Lu S, Chen X, Wu Y, He P, Zhang X, Chen H, Wang H, and Gao Y

Subjects

Reference Values, China, Laboratory Proficiency Testing, Reference Standards, Food, Genetically Modified, Zea mays genetics, Zea mays chemistry, Plants, Genetically Modified genetics, Plants, Genetically Modified chemistry

Abstract

The Asia Pacific Metrology Program and the Accreditation Cooperation joint Proficiency Testing (PT) program for the quantification of genetically modified maize MON87427 was organized by the National Institute of Metrology, China, to enhance the measurement accuracy and metrological traceability in the region. Certified reference materials were employed as test samples; metrologically traceable certified reference values served as PT reference values (PTRVs) for evaluating the participants results. The consensus values obtained from the participants were higher than the assigned values, potentially due to the systematic effects of DNA extraction process. The participants' relatively poor overall performance by the ζ-score compared with z-score demonstrates their need to thoroughly investigate quantification bias to elevate the measurement capability of genetically modified (GM) content and deepen their understanding of uncertainty estimation. This program confirmed the importance of using metrologically traceable reference values instead of consensus values as PTRV for reliable performance assessment., Competing Interests: Declaration of competing interest The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2024 Elsevier Ltd. All rights reserved.)

Published

2024

16. Whole-genome sequencing for antimicrobial surveillance: species-specific quality thresholds and data evaluation from the network of the European Union Reference Laboratory for Antimicrobial Resistance genomic proficiency tests of 2021 and 2022.

Author

Sørensen LH, Pedersen SK, Jensen JD, Lacy-Roberts N, Andrea A, S M Brouwer M, Veldman KT, Lou Y, Hoffmann M, and S Hendriksen R

Subjects

Humans, Quality Control, Bacteria genetics, Bacteria drug effects, Anti-Bacterial Agents pharmacology, Laboratories standards, Species Specificity, Whole Genome Sequencing standards, European Union, Laboratory Proficiency Testing, Drug Resistance, Bacterial genetics, Genome, Bacterial

Abstract

As antimicrobial resistance (AMR) surveillance shifts to genomics, ensuring the quality of whole-genome sequencing (WGS) data produced across laboratories is critical. Participation in genomic proficiency tests (GPTs) not only increases individual laboratories' WGS capacity but also provides a unique opportunity to improve species-specific thresholds for WGS quality control (QC) by repeated resequencing of distinct isolates. Here, we present the results of the EU Reference Laboratory for Antimicrobial Resistance (EURL-AR) network GPTs of 2021 and 2022, which included 25 EU national reference laboratories (NLRs). A total of 392 genomes from 12 AMR-bacteria were evaluated based on WGS QC metrics. Two percent ( n = 9) of the data were excluded, due to contamination, and 11% ( n = 41) of the remaining genomes were identified as outliers in at least one QC metric and excluded from computation of the adjusted QC thresholds (AQT). Two QC metric correlation groups were identified through linear regression. Eight percent ( n = 28) of the submitted genomes, from 11 laboratories, failed one or more of the AQTs. However, only three laboratories (12%) were identified as underperformers, failing across AQTs for uncorrelated QC metrics in at least two genomes. Finally, new species-specific thresholds for "N50" and "number of contigs > 200 bp" are presented for guidance in routine laboratory QC. The continued participation of NRLs in GPTs will reveal WGS workflow flaws and improve AMR surveillance data. GPT data will continue to contribute to the development of reliable species-specific thresholds for routine WGS QC, standardizing sequencing data QC and ensure inter- and intranational laboratory comparability.IMPORTANCEIllumina next-generation sequencing is an integral part of antimicrobial resistance (AMR) surveillance and the most widely used whole-genome sequencing (WGS) platform. The high-throughput, relative low-cost, high discriminatory power, and rapid turnaround time of WGS compared to classical biochemical methods means the technology will likely remain a fundamental tool in AMR surveillance and public health. In this study, we present the current level of WGS capacity among national reference laboratories in the EU Reference Laboratory for AMR network, summarizing applied methodology and statistically evaluating the quality of the obtained sequence data. These findings provide the basis for setting new and revised thresholds for quality metrics used in routine WGS, which have previously been arbitrarily defined. In addition, underperforming participants are identified and encouraged to evaluate their workflows to produce reliable results., Competing Interests: The authors declare no conflict of interest.

Published

2024

17. Challenges and improvements in HER2 scoring and histologic evaluation: insights from a national proficiency testing scheme for breast cancer diagnosis in China.

Author

Xue X, Guo L, Guo C, Xu L, Li L, Yang L, Wang X, Rao W, Yuan P, Mu J, Li J, Wang B, Zhou Q, Xue W, Ma F, Yang W, and Ying J

Subjects

Humans, Female, China, In Situ Hybridization, Fluorescence standards, Biomarkers, Tumor, Pathologists, Breast Neoplasms diagnosis, Breast Neoplasms pathology, Breast Neoplasms metabolism, Receptor, ErbB-2 metabolism, Laboratory Proficiency Testing

Abstract

Background: In 2022, our team launched the pioneering national proficiency testing (PT) scheme for the pathological diagnosis of breast cancer, rapidly establishing its credibility throughout China. Aiming to continuously monitor and improve the proficiency of Chinese pathologists in breast pathology, the second round of the PT scheme was initiated in 2023, which will expand the number of participating institutions, and will conduct a nationwide investigation into the interpretation of HER2 0, 1+, and 2+/FISH- categories in China., Methods: The methodology employed in the current round of PT scheme closely mirrors that of the preceding cycle in 2022, which is designed and implemented according to the "Conformity assessment-General requirements for proficiency testing"(GB/T27043-2012/ISO/IEC 17043:2010). More importantly, we utilized a statistics-based method to generate assigned values to enhance their robustness and credibility., Results: The final PT results, published on the website of the National Quality Control Center for Cancer ( http://117.133.40.88:3927 ), showed that all participants passed the testing. However, a few institutions demonstrated systemic biases in scoring HER2 0, 1+, and 2+/FISH- with accuracy levels below 59%, considered unsatisfactory. Especially, the concordance rate for HER2 0 cases was only 78.1%, indicating challenges in distinguishing HER2 0 from low HER2 expression. Meanwhile, areas for histologic type and grade interpretation improvement were also noted., Conclusions: Our PT scheme demonstrated high proficiency in diagnosing breast cancer in China. But it also identified systemic biases in scoring HER2 0, 1+, and 2+/FISH- at some institutions. More importantly, our study highlighted challenges in the evaluation at the extreme lower end of the HER2 staining spectrum, a crucial area for further research. Meanwhile, it also revealed the need for improvements in interpreting histologic types and grades. These findings strengthened the importance of robust quality assurance mechanisms, like the nationwide PT scheme conducted in this study, to maintain high diagnostic standards and identify areas requiring further training and enhancement., (© 2024. The Author(s).)

Published

2024

18. Proficiency Testing Customization in Clinical Trials: How the pSMILE Project Ensures High-Quality Proficiency Testing Coverage for International Laboratories.

Author

Leach A, Murphy KJ, Godard M, Schwartz M, and Sokoll LJ

Subjects

Humans, Laboratories, Clinical, Laboratories standards, Laboratory Proficiency Testing, Clinical Trials as Topic

Published

2024

19. The Critical Need to Expand Proficiency Testing to Cover Telepathology.

Author

Petersen J, Jhala N, and Jhala D

Subjects

Humans, Laboratory Proficiency Testing, Pathology, Clinical methods, Pathology, Clinical standards, Telepathology

Abstract

Competing Interests: The authors have no relevant financial interest in the products or companies described in this article.

Published

2024

20. High success rate of first proficiency testing for RET fusions and RET mutations in lung and thyroid cancer samples by various methods.

Author

Siebolts U, Pappesch R, Bauer M, Dietmaier W, Ernst M, Haak A, Hartmann N, Ilm K, Kalbourtzis S, Krause T, Kazdal D, Schorle H, Utpatel K, and Merkelbach-Bruse S

Subjects

Humans, Laboratory Proficiency Testing, Carcinoma, Non-Small-Cell Lung genetics, Carcinoma, Non-Small-Cell Lung diagnosis, Reproducibility of Results, DNA Mutational Analysis methods, Gene Fusion, In Situ Hybridization methods, Proto-Oncogene Proteins c-ret genetics, Thyroid Neoplasms genetics, Thyroid Neoplasms pathology, Thyroid Neoplasms diagnosis, Lung Neoplasms genetics, Lung Neoplasms diagnosis, Lung Neoplasms pathology, Mutation, Carcinoma, Neuroendocrine genetics, Carcinoma, Neuroendocrine pathology, Carcinoma, Neuroendocrine diagnosis, High-Throughput Nucleotide Sequencing

Abstract

This study describes the external quality assessment (EQA) scheme for molecular testing of RET alterations in non-small cell lung cancer (NSCLC), medullary thyroid carcinomas (MTC), and non-MTC. The lead panel institute and Quality Assurance Initiative in Pathology (Qualitätssicherungs-Initiative Pathologie [QuIP] GmbH) selected formalin-fixed paraffin-embedded (FFPE) tissue from MTC for RET mutation testing by next-generation sequencing (NGS) methods and FFPE tissue from NSCLC and non-MTC for RET gene fusion testing using either in situ hybridisation (ISH) or NGS methods, forming 3 sub-schemes of the EQA scheme. Tissue material underwent an internal validation phase followed by an external testing phase. The internal validation phase served as a cross-validation step conducted by panel institutes. In the external testing phase, the number of participating institutes in the RET point mutation sub-scheme, RET fusion (ISH) sub-scheme, and RET fusion (NGS) sub-scheme was 32, 24, and 38, respectively. The reported success rates for external testing were 96.0%, 89.5%, and 93.5% for the RET point mutation, the ISH RET fusion, and the NGS RET fusion EQA sub-schemes, respectively. These findings confirm the reliability of the NGS method in detecting RET alterations and align with current screening recommendations. Overall, 31 institutes were certified for RET point mutation testing by NGS methods, 22 institutes were certified for RET fusion testing by ISH, and 36 institutes were certified for RET fusion testing by NGS methods. Results can be employed to inform real-world diagnostic decisions in Germany, Austria, and Switzerland., (© 2024. The Author(s), under exclusive licence to Springer-Verlag GmbH Germany, part of Springer Nature.)

Published

2024

21. Anti-Rubella Immunoglobulin G Proficiency Testing Results Suggest Consistent Manufacturer Differences and Opportunity for Harmonization.

Author

Treger RS, Long TC, Calvey SL, Tacker DH, Kadkhoda K, Wener MH, and Fink SL

Subjects

Humans, Laboratory Proficiency Testing, Immunoglobulin G blood, Immunoglobulin G analysis

Published

2024

22. Continued improvement in the development of the SARS-CoV-2 whole genome sequencing proficiency testing program.

Author

Lau KA, Foster CSP, Theis T, Draper J, Sullivan MJ, Ballard S, and Rawlinson WD

Subjects

Humans, New Zealand, Australia, Genome, Viral genetics, Whole Genome Sequencing, SARS-CoV-2 genetics, COVID-19 diagnosis, COVID-19 virology, Laboratory Proficiency Testing

Abstract

Application of whole genome sequencing (WGS) has allowed monitoring of the emergence of variants of concern (VOC) of severe acute respiratory syndrome-related coronavirus 2 (SARS-CoV-2) globally. Genomic investigation of emerging variants and surveillance of clinical progress has reduced the public health impact of infection during the COVID-19 pandemic. These steps required developing and implementing a proficiency testing program (PTP), as WGS has been incorporated into routine reference laboratory practice. In this study, we describe how the PTP evaluated the capacity and capability of one New Zealand and 14 Australian public health laboratories to perform WGS of SARS-CoV-2 in 2022. The participants' performances in characterising a specimen panel of known SARS-CoV-2 isolates in the PTP were assessed based on: (1) genome coverage, (2) Pango lineage, and (3) sequence quality, with the choice of assessment metrics refined based on a previously reported assessment conducted in 2021. The participants' performances in 2021 and 2022 were also compared after reassessing the 2021 results using the more stringent metrics adopted in 2022. We found that more participants would have failed the 2021 assessment for all survey samples and a significantly higher fail rate per sample in 2021 compared to 2022. This study highlights the importance of choosing appropriate performance metrics to reflect better the laboratories' capacity to perform SARS-CoV-2 WGS, as was done in the 2022 PTP. It also displays the need for a PTP for WGS of SARS-CoV-2 to be available to public health laboratories ongoing, with continuous refinements in the design and provision of the PTP to account for the dynamic nature of the COVID-19 pandemic as SARS-CoV-2 continues to evolve., (Copyright © 2024 Royal College of Pathologists of Australasia. Published by Elsevier B.V. All rights reserved.)

Published

2024

23. Prevalence of Syphilis Serology Testing Algorithm Among Laboratory Participants in the College of American Pathologists Proficiency Testing Program.

Author

Kadkhoda K, Souers RJ, and Calvey SL

Subjects

Humans, Pathologists, United States epidemiology, Prevalence, Syphilis diagnosis, Syphilis epidemiology, Syphilis blood, Laboratory Proficiency Testing, Algorithms, Syphilis Serodiagnosis methods

Published

2024

24. Sources of variability in Luminex bead-based cytokine assays: Evidence from twelve years of multi-site proficiency testing.

Author

Rountree W, Lynch HE, Denny TN, Sempowski GD, and Macintyre AN

Subjects

Humans, Reproducibility of Results, Quality Control, Immunoassay methods, Immunoassay standards, United States, Biomarkers blood, Cytokines blood, Laboratory Proficiency Testing

Abstract

Bead array assays, such as those sold by Luminex, BD Biosciences, Sartorius, Abcam and other companies, are a well-established platform for multiplexed quantification of cytokines and other biomarkers in both clinical and discovery research environments. In 2011, the National Institute of Allergy and Infectious Diseases (NIAID)-funded External Quality Assurance Program Oversight Laboratory (EQAPOL) established a proficiency assessment program to monitor participating laboratories performing multiplex cytokine measurements using Luminex bead array technology. During every assessment cycle, each site was sent an assay kit, a protocol, and blinded samples of human sera spiked with recombinant cytokines. Site results were then evaluated for performance relative to peer laboratories. After over a decade of biannual assessments, the cumulative dataset contained over 15,500 bead array observations collected at more than forty laboratories in twelve countries. These data were evaluated alongside post-assessment survey results to empirically test factors that may contribute to variability and accuracy in Luminex bead-based cytokine assays. Bead material, individual technical ability, analyte, analyte concentration, and assay kit vendor were identified as significant contributors to assay performance. In contrast, the bead reader instrument model and the use of automated plate washers were found not to contribute to variability or accuracy, and sample results were found to be highly-consistent between assay kit-manufacturing lots and over time. In addition to these statistical analyses, subjective evaluations identified technical ability, instrument failure, protocol adherence, and data transcription errors as the most common causes of poor performance in the proficiency program. The findings from the EQAPOL multiplex program were then used to develop recommended best practices for bead array monitoring of human cytokines. These included collecting samples to assay as a single batch, centralizing analysis, participating in a quality assurance program, and testing samples using paramagnetic-bead kits from a single manufacturer using a standardized protocol., Competing Interests: Declaration of competing interest The authors have no competing interests to declare., (Copyright © 2023. Published by Elsevier B.V.)

Published

2024

25. Low utilization of epidemiological cutoff values to interpret in vitro antifungal susceptibility testing among clinical laboratory participants in two College of American Pathologists (CAP) proficiency testing programs.

Author

Sullivan KV, Long T, Hillesland E, Rhoads DD, Wojewoda CM, and Zhang SX

Subjects

Humans, United States, Mycoses microbiology, Antifungal Agents pharmacology, Microbial Sensitivity Tests standards, Laboratory Proficiency Testing

Abstract

Competing Interests: The authors declare no conflict of interest.

Published

2024

26. Implementation, Evolution, and Laboratory Performance of Methods-Based Proficiency Testing for Next-Generation Sequencing Detection of Germline Sequence Variants.

Author

Tsuchiya KD, Funke B, Hegde M, Santani A, Souers RJ, Szelinger S, Halley J, Zhao Q, Mot N, Roy A, Smith VL, Zhang BM, Voelkerding K, and Moyer AM

Subjects

Humans, Genetic Testing methods, Genetic Testing standards, Laboratories, Clinical, Laboratory Proficiency Testing, High-Throughput Nucleotide Sequencing standards, High-Throughput Nucleotide Sequencing methods, Germ-Line Mutation

Abstract

Context.—: Next-generation sequencing (NGS)-based assays are used for diagnosis of diverse inherited disorders. Limited data are available pertaining to interlaboratory analytical performance of these assays., Objective.—: To report on the College of American Pathologists (CAP) NGS Germline Program, which is methods based, and explore the evolution in laboratory testing practices., Design.—: Results from the NGS Germline Program from 2016-2020 were analyzed for interlaboratory analytical performance. Self-reported laboratory testing practices were also evaluated., Results.—: From 2016-2020, a total of 297 laboratories participated in at least 1 program mailing. Of the 289 laboratories that provided information on tests offered, 138 (47.8%) offered only panel testing throughout their enrollment, while 35 (12.1%) offered panels and exome testing, 30 (10.4%) offered only exomes, 9 (3.1%) offered only genomes, and 15 (5.2%) offered panels, exomes, and genomes. The remainder (62 laboratories, 21.4%) changed their test offerings during the 2016-2020 timeframe. Considering each genomic position/interval, the median detection percentage at variant positions across the 2016-2020 mailings ranged from 94.3% to 100%, while at reference positions (no variant detected), the median correct response percentage was 100% across all mailings. When considering performance of individual laboratories, 89.5% (136 of 152) to 98.0% (149 of 152) of laboratories successfully met the detection threshold (≥90% of the variants present), while 94.6% (87 of 92) to 100% (163 of 163) of laboratories met the 95% specificity threshold across mailings., Conclusions.—: Since the inception of this program, laboratories have consistently performed well. The median sensitivity and specificity of detection of sequence variants included in this program (eg, single nucleotide variants, insertions, and deletions) were 100.0%., (© 2024 College of American Pathologists.)

Published

2024

27. Diagnosis of von Willebrand disease: An assessment of the quality of testing in North American laboratories.

Author

Abdulrehman, Jameel, Ziemba, Yonah C., Hsu, Peihong, Van Cott, Elizabeth M., Plumhoff, Elizabeth A., Meijer, Piet, Hollestelle, Martine J., and Selby, Rita

Subjects

*VON Willebrand disease, *VON Willebrand factor, *BLOOD coagulation disorders, *BLOOD coagulation factor VIII, *CLINICAL pathology, *GAUSSIAN distribution

Abstract

Background: Laboratory diagnosis of von Willebrand Disease (VWD) is complex. Reliance on laboratory testing can be problematic as different VWD screening panels, assays and methodologies can produce analytic variability in test results. Objectives: To compare the degree of imprecision among the VWD assays and within the platelet binding activity (PBA) assays, to determine the consensus among the VWD assays for correct classification of sample results, and to determine consensus among laboratories' von Willebrand factor (VWF) multimer interpretations and final interpretations of the VWD panels. Patients/Methods: Proficiency testing results from the North American Specialized Coagulation Laboratory Association (NASCOLA) submitted by laboratories from 2010 to 2019 for all normal, type (T) 1 VWD and T2 VWD samples were analysed. Results and Conclusions: Imprecision was lowest for VWF antigen and highest for collagen binding activity (CBA) with median coefficient of variation (CV) of 12% (interquartile range (IQR) 7%) and 23% (IQR 21%) respectively. Within the VWF PBA assays, the gain‐of‐function mutant GP1b binding (VWF: GP1bM) methods had the least imprecision (CV 9%, IQR 10%). All assays, including the various PBA methods had excellent consensus. The majority of laboratories agreed that normal (median consensus‐82%, IQR 16%) and T1 VWD (median consensus‐100%, IQR 9%) samples had normal multimer distribution. Consensus among laboratories for final interpretations was excellent for normal samples (median 81%, IQR 8%), good for T1 VWD samples (median 59%, IQR 9%), and fair for T2 VWD samples (median 44%, IQR 21%). Consensus on final interpretation decreased as sample complexity increased. [ABSTRACT FROM AUTHOR]

Published

2021

28. Sequence Variation in Amplification Target Genes and Standards Influences Interlaboratory Comparison of BK Virus DNA Load Measurement.

Author

Solis, Morgane, Meddeb, Mariam, Sueur, Charlotte, Domingo-Calap, Pilar, Soulier, Eric, Chabaud, Angeline, Perrin, Peggy, Moulin, Bruno, Bahram, Seiamak, Stoll-Keller, Françoise, Caillard, Sophie, Barth, Heidi, and Fafi-Kremer, Samira

Subjects

BK Virus, DNA, Viral, France, Genetic Variation, Hospitals, Humans, Laboratory Proficiency Testing, Polyomavirus Infections, Sensitivity and Specificity, Viral Load

Abstract

International guidelines define a BK virus (BKV) load of ≥4 log10 copies/ml as presumptive of BKV-associated nephropathy (BKVN) and a cutoff for therapeutic intervention. To investigate whether BKV DNA loads (BKVL) are comparable between laboratories, 2 panels of 15 and 8 clinical specimens (urine, whole blood, and plasma) harboring different BKV genotypes were distributed to 20 and 27 French hospital centers in 2013 and 2014, respectively. Although 68% of the reported results fell within the acceptable range of the expected result ±0.5 log10, the interlaboratory variation ranged from 1.32 to 5.55 log10. Polymorphisms specific to BKV genotypes II and IV, namely, the number and position of mutations in amplification target genes and/or deletion in standards, arose as major sources of interlaboratory disagreements. The diversity of DNA purification methods also contributed to the interlaboratory variability, in particular for urine samples. Our data strongly suggest that (i) commercial external quality controls for BKVL assessment should include all major BKV genotypes to allow a correct evaluation of BKV assays, and (ii) the BKV sequence of commercial standards should be provided to users to verify the absence of mismatches with the primers and probes of their BKV assays. Finally, the optimization of primer and probe design and standardization of DNA extraction methods may substantially decrease interlaboratory variability and allow interinstitutional studies to define a universal cutoff for presumptive BKVN and, ultimately, ensure adequate patient care.

Published

2015

29. Design and Implementation of an External Quality Assessment Program for HIV Viral Load Measurements Using Dried Blood Spots

Author

Prach, Lisa M, Puren, Adrian, Lippman, Sheri A, Carmona, Sergio, Stephenson, Sophie, Cutler, Ewalde, Barnhart, Scott, and Liegler, Teri

Subjects

Medical Microbiology, Biomedical and Clinical Sciences, Infectious Diseases, Clinical Research, Sexually Transmitted Infections, HIV/AIDS, Infection, Blood, HIV Infections, HIV-1, Humans, Laboratory Proficiency Testing, Quality Assurance, Health Care, RNA, Viral, Viral Load, Biological Sciences, Agricultural and Veterinary Sciences, Medical and Health Sciences, Microbiology, Clinical sciences, Medical microbiology

Abstract

An external quality assurance program was developed for HIV-1 RNA viral load measurements taken from dried blood spots using a reference panel and field-collected specimens. The program demonstrated that accurate and reproducible quantitation can be obtained from field-collected specimens. Residual proviral DNA may confound interpretation in virologically suppressed subjects.

Published

2015

30. Audit of sweat chloride testing reveals analytical errors.

Author

Prenzel, Freerk, Ceglarek, Uta, Adams, Ines, Hammermann, Jutta, Issa, Ulrike, Lohse, Gerhild, Mainz, Jochen G., Meister, Jochen, Spittel, Dana, Thoss, Karin, Vogel, Mandy, Duckstein, Franziska, Henn, Constance, and Hentschel, Julia

Subjects

*STANDARD operating procedure, *CHLORIDES, *CYSTIC fibrosis, *BIOMARKERS, *QUALITY assurance

Abstract

Sweat chloride testing (SCT) is the mainstay for the diagnosis of cystic fibrosis (CF) and biomarker in the evaluation of CFTR-modifying drugs. To be a reliable and valid tool, analytical variance (CVA) must be minimized. However, external quality assessments have revealed significant deviations in routine clinical practice. Our goal was to identify and quantify technical errors through proficiency testing and simulations. Chloride concentrations of three blinded samples (each as triplicates) were measured in 9 CF centers using a chloridometer in a routine setting. Technical errors were simulated and quantified in a series of measurements. We compared imprecision and bias before and after a counseling session by evaluating coefficients of variation (CV), adherence to tolerance limits, and inter-rater variability coefficients. Pipetting errors resulting in changes in sample volume were identified as the main source of error with deviations up to 41%. After the counseling session, the overall CVA decreased from 7.6 to 5.2%, the pass rate increased from 67 to 92%, and the inter-rater variability diminished. Significant deviations continued to be observed in individual centers. Prevention of technical errors in SCT decreases imprecision and bias. Quality assurance programs must be established in all CF centers, including staff training, standard operating procedures, and proficiency testing. [ABSTRACT FROM AUTHOR]

Published

2021

31. A pilot external quality assurance study of transfusion screening for HIV, HCV and HBsAG in 12 African countries

Author

Bloch, EM, Shah, A, Kaidarova, Z, Laperche, S, Lefrere, J‐J, Hasselt, J, Zacharias, P, Murphy, EL, and Group, the Anglophone Africa Transfusion Research

Subjects

Medical Microbiology, Biomedical and Clinical Sciences, Clinical Sciences, Prevention, Digestive Diseases, Infectious Diseases, Liver Disease, Clinical Research, HIV/AIDS, Emerging Infectious Diseases, Hepatitis, Hepatitis - C, Infection, Good Health and Well Being, Africa, Antibodies, Viral, Antigens, Viral, Blood Safety, Blood Transfusion, Donor Selection, HIV Infections, Hepatitis B, Hepatitis B Surface Antigens, Hepatitis C, Humans, Immunoenzyme Techniques, Laboratories, Pilot Projects, Quality Assurance, Health Care, Sensitivity and Specificity, blood transfusion, hepatitis B surface antigens, hepatitis C antibodies, HIV, laboratory proficiency testing, Anglophone Africa Transfusion Research Group, Blood transfusion, Hepatitis B surface antigens, Hepatitis C antibodies, Laboratory proficiency testing, Medical Physiology, Cardiovascular System & Hematology, Clinical sciences

Abstract

Background and objectivesSerologic screening for the major transfusion transmissible viruses (TTV) is critical to blood safety and has been widely implemented. However, actual performance as measured by proficiency testing has not been well studied in sub-Saharan Africa. Therefore, we conducted an external quality assessment of laboratories engaged in transfusion screening in the region.Materials and methodsBlinded test panels, each comprising 25 serum samples that were pedigreed for HIV, HBsAg, HCV and negative status, were sent to participating laboratories. The panels were tested using the laboratories' routine donor screening methods and conditions. Sensitivity and specificity were calculated, and multivariable analysis was used to compare performance against mode of testing, country and infrastructure.ResultsA total of 12 African countries and 44 laboratories participated in the study. The mean (range) sensitivities for HIV, HBsAg and HCV were 91·9% (14·3-100), 86·7% (42·9-100) and 90·1% (50-100), respectively. Mean specificities for HIV, HBsAg and HCV were 97·7%, 97% and 99·5%, respectively. After adjusting for country and infrastructure, rapid tests had significantly lower sensitivity than enzyme immunoassays for both HBsAg (P

Published

2014

32. False-Positive Papanicolaou (PAP) Test Rates in the College of American Pathologists PAP Education and PAP Proficiency Test Programs: Evaluation of False-Positive Responses of High-Grade Squamous Intraepithelial Lesion or Cancer to a Negative Reference Diagnosis

Author

Crothers, Barbara A, Booth, Christine Noga, Darragh, Teresa Marie, Zhao, Chengquan, Souers, Rhona J, Thomas, Nicole, and Moriarty, Ann T

Subjects

Cancer, Quality Education, Carcinoma, Squamous Cell, Diagnostic Errors, False Positive Reactions, Female, Humans, Incidence, Laboratory Proficiency Testing, Papanicolaou Test, Pathology, Clinical, Professional Competence, Reference Standards, Retrospective Studies, Time Factors, Uterine Cervical Neoplasms, Uterine Cervical Dysplasia, Clinical Sciences, Pathology

Abstract

ContextIn cytology proficiency testing (PT), participants fail for incorrectly interpreting a high-grade squamous intraepithelial lesion or cancer (HSIL+) Papanicolaou test result as negative. This penalty may lead to a false-positive interpretation of negative slides as HSIL+ to avoid failure.ObjectiveTo investigate factors related to false-positive responses in a PT versus an educational environment.DesignWe analyzed 420,079 responses from 9414 validated negative reference slides in the College of American Pathologists Interlaboratory Comparison Program in Gynecologic Cytopathology (PAP Education) and compared them with responses from the Gynecologic Cytology Proficiency Testing Program for the percentage of false-positive (HSIL+) interpretations in each of 7 negative subcategories. We evaluated the influence of preparation type (ThinPrep, SurePath, and conventional Papanicolaou test), participant type (pathologist or cytotechnologist), and program time interval (preproficiency test or PT) on a false-positive response.ResultsReference diagnosis and participant type, but not preparation type, were statistically correlated to false-positive responses. The interaction between program time interval and participant type was also significant. Pathologists had higher rates of false-positive results on preproficiency test (1.2% [800 of 68,690]) than they did on PT (0.8% [993 of 129,857]). Cytotechnologists had no differences between program time intervals (preproficiency, 0.9% [515 of 63,281] versus PT, 1.0 [1231 of 121,621]; P = .91). Negative subcategories frequently mistaken for HSIL+ were reparative changes (4.7% [427 of 9069]), atrophic vaginitis (1.8% [18 of 987]), and negative for intraepithelial lesion or malignancy (1.2% [2143 of 178,651]), but during PT, false-positive rates were significantly increased only for the negative for intraepithelial lesion or malignancy and herpes simplex virus (P < .001).ConclusionsPathologists had lower false-positive rates in the Gynecologic Cytology Proficiency Testing Program than they did in PAP Education, but participants were more likely to report a false-positive response (HSIL+) for negative for intraepithelial lesion or malignancy and herpes simplex virus in the Gynecologic Cytology Proficiency Test Program.

Published

2014

33. Diphtheria diagnostic capacity in the Western Pacific Region

Author

Santosh Gurung, Amy Trindall, Lucy Reeve, Adroulla Efstratiou, and Varja Grabovac

Subjects

bacteriological techniques/methods, corynebacterium infections/microbiology, laboratory proficiency testing, Medicine, Public aspects of medicine, RA1-1270

Abstract

Diphtheria is an acute infectious disease affecting the upper respiratory tract and occasionally the skin and is caused by the action of diphtheria toxin produced by Corynebacterium diphtheriae, Corynebacterium ulcerans and Corynebacterium pseudotuberculosis. Corynebacterium infections are usually difficult to control due to their epidemic patterns, the emergence of new strains, novel reservoirs and their dissemination to susceptible human and animal populations.1 Although C. diphtheriae is largely controlled through mass immunization programmes, diphtheria escalated to epidemic proportions within the Russian Federation and the former Soviet Republics in the 1990s, highlighting the potential for this disease to cause morbidity and mortality when immunization programmes are disrupted.2 A recent review of global diphtheria epidemiology, which included an analysis of cases and information about age, showed age distribu­tion shifts and found that the majority of cases occur in adoles­cents and adults.3 Shifts in age distribution, from children to adolescents and adults, were observed from countries in the Western Pacific Region such as the Lao People’s Democratic Republic,4 the Philippines3 and Viet Nam.5

Published

2019

34. First inter-laboratory comparison of Echinococcus granulosus sensu lato diagnosis in Latin America

Author

María Isabel Jercic, Graciela Santillan, Susana Elola, William Quispe Paredes, Lidia B. Conza Blanco, Noelia Morel, Rodrigo Villegas, Baldomero Molina Flores, Cesar M. Gavidia, Marta Cabrera, Alexandre Guerra dos Santos, Manuel J. Sanchez-Vazquez, Melody J. Maxwell, Marco A. Vigilato, Edmundo Larrieu, and Víctor J. Del Rio Vilas

Subjects

echinococcosis, dog diseases, laboratory proficiency testing, south america, Medicine, Arctic medicine. Tropical medicine, RC955-962, Public aspects of medicine, RA1-1270

Abstract

Objective. To compare the performance of polymerase chain reaction (PCR) and enzyme-linked immunosorbent assay (ELISA) tests for diagnosing Echinococcus granulosus in dog feces among national reference laboratories in Argentina, Chile, Peru, and Uruguay. Methods. National laboratories affiliated with the Ministry of Health/Agriculture of each country exchanged panels of 10 positive/negative samples obtained from their regular national surveillance programs in November 2015 – November 2016. All laboratories applied PCR; two also applied ELISA techniques. Sensitivity and specificity were determined for each laboratory and concordance of results among the laboratories was evaluated by Cohen Kappa coefficient. Results. Poor concordance (3 of 10 paired comparisons had values of Kappa > 0.4), low sensitivity and specificity across all laboratories, and poor performance of both techniques in detecting E. granulosus in canine feces was demonstrated in this study. An ex-post comparison of the laboratories’ test protocols showed substantial heterogeneity that could partially explain poor concordance of results. Conclusion. The results underscore the heterogeneity of canine echinococcosis diagnosis across the region and indicate possible sources of variability. Efforts to standardize canine echinococcosis testing must be included in the plan of action for the Regional Initiative for the Control of Cystic Echinococcosis. Future comparisons with fecal samples of known parasite load are needed.

Published

2019

35. Forensische DNA-Methylierungsanalyse: Zweiter, technischer Ringversuch der Arbeitsgruppe „Molekulare Altersschätzung" der Deutschen Gesellschaft für Rechtsmedizin.

Author

Naue, Jana, Pfeifer, Manuel, Augustin, Christa, Becker, Julia, Fleckhaus, Jan, Grabmüller, Melanie, Han, Yang, Heidorn, Frank, Hollaender, Olivia, Klein-Unseld, Rachel, Kulstein, Galina, Lichtenwald, Julia, Neubauer, Jacqueline, Suarez, Philippe, Haas, Cordula, Schneider, Peter M., Vennemann, Marielle, Böhme, Petra, and Arbeitsgemeinschaft Molekulare Altersschätzung der Deutschen Gesellschaft für Rechtsmedizin (DGRM)

Abstract

Copyright of Rechtsmedizin is the property of Springer Nature and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published

2021

36. Forensische DNA-Methylierungsanalyse: Erster, technischer Ringversuch der Arbeitsgruppe „Molekulare Altersschätzung" der Deutschen Gesellschaft für Rechtsmedizin.

Author

Holländer, Olivia, Schwender, Kristina, Böhme, Petra, Fleckhaus, Jan, Haas, Cordula, Han, Yang, Heidorn, Frank, Klein-Unseld, Rachel, Lichtenwald, Julia, Naue, Jana, Neubauer, Jacqueline, Poetsch, Micaela, Schneider, Peter M., Wagner, Wolfgang, Vennemann, Marielle, and Arbeitsgemeinschaft Molekulare Altersschätzung der Deutschen Gesellschaft für Rechtsmedizin (DGRM)

Abstract

Copyright of Rechtsmedizin is the property of Springer Nature and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published

2021

37. Comparison of the Results of Proficiency Testing in Seven Medical Laboratories - a Benchmark Project to Define a Uniform Key Performance Indicator.

Author

Ioculano, Martin, Occhipinti, Francesca, Tumiatti, Daniel, Platzgummer, Stefan, Troi, Christina, Wierer, Brigitte, and Mueller, Thomas

Subjects

MEDICAL laboratories, KEY performance indicators (Management), ABILITY

Abstract

Background: In medical laboratories, it is mandatory to ensure the analytical quality of the measurement procedures by proficiency testing (PT). The aim of this study was to evaluate whether the PT results of seven medical laboratories in South Tyrol - as a measure of the analytical performance - were different. Methods: As a measure for the analytical performance of the individual laboratories, we used the PT results (RIQAS, Randox international quality assessment scheme) of one year for 34 analytes. We calculated annual 'total scores' of each analyte for all participating laboratories and compared them statistically. Results: In 2018, there was a highly significant difference between the seven laboratories in the 'total scores' for the 34 analytes (p < 0.001). The laboratories had a 'cumulative, annual total score' of 75 - 91% of the maximum achievable values. Essentially, two groups could be distinguished. Laboratories 1 - 3 achieved better results (90 - 91%) than laboratories 4 - 7 (77 - 82%). In particular, the non-participation of the laboratories 4 - 7 in several PT cycles in 2018 and the registration in the wrong homogeneous group for some analytes in the laboratories 4 and 5 seem to be responsible for the worse results. Conclusions: The analytical performance as assessed by the PT results was different across the seven participating laboratories of the South Tyrolean Medical Service. Based on our study results, we defined a uniform key performance indicator for the seven laboratories with a limit value for the 'cumulative, annual total score' of > 80%. [ABSTRACT FROM AUTHOR]

Published

2021

38. Identification of Trichomonas vaginalis in Different Papanicolaou Test Preparations: Trends Over Time in the College of American Pathologists Educational Interlaboratory Comparison Program

Author

Howell, Lydia Pleotis, Darragh, Teresa M, Souers, Rhona J, Thomas, Nicole, and Moriarty, Ann T

Subjects

Clinical Research, Female, Humans, Laboratory Proficiency Testing, Nonlinear Dynamics, Papanicolaou Test, Pathology, Clinical, Societies, Medical, Trichomonas vaginalis, United States, Vaginal Smears, Clinical Sciences, Pathology

Abstract

ContextThe College of American Pathologists' Interlaboratory Comparison Program in Gynecologic Cytology has seen an increase in enrollment in liquid-based Papanicolaou test challenges with a decrease for conventional Papanicolaou tests. Trichomonas vaginalis can be difficult to identify in all preparation types.ObjectivesTo evaluate 20 years of participant results from the College of American Pathologists Interlaboratory Comparison Program in Gynecologic Cytology for Trichomonas to ascertain whether performance has changed because of the introduction of liquid-based Papanicolaou and proficiency testing.DesignConcordance rates for the target diagnosis of Trichomonas vaginalis were evaluated for 167,956 participant responses (1990-2010). A nonlinear mixed model was fit with participant type, preparation type, and a 2-level program year (1990-2005 and 2006-2010) reflecting before and after proficiency testing began. A repeated-measures component allowed modeling of the slide-specific performance to ensure that the overall results were not based on the performance of a few slides.ResultsCytotechnologists had higher concordance with the target diagnosis than did pathologists (89.8% [72,992 of 81,319] versus 83.4% [72,271 of 86,637], P < .001) and better performance for each preparation type (P = .003). Concordance initially dropped after the introduction of proficiency testing (P < .001) for conventional and liquid-based (SurePath) preparations by both participant types, followed by quick, parallel improvement.ConclusionsPerformance is high in the detection of Trichomonas vaginalis in the College of American Pathologists Interlaboratory Comparison Program in Gynecologic Cytology. Liquid-based Papanicolaou and proficiency testing minimally affected participant performance. Cytotechnologists performed better over time and across preparation types than did pathologists, although pathologists showed performance results parallel to that of the cytotechnologists. Awareness of the performance differences by pathologists and cytotechnologists, as well as their difference in proficiency among liquid-based techniques, may help ensure accurate results in clinical practice.

Published

2013

39. The development and implementation of a proficiency testing program for SARS-CoV-2 using dried tube specimens in resource-limited countries.

Author

Lutaaya P, Guido O, Ssentamu HN, Kasule GW, Akumu M, Kabahita JM, Bagaya B, Musisi K, Oola D, Katuramu A, Nsawotebba A, Kigozi E, Nakazzi F, Solomon JK, Adam I, Beatrice O, Namutebi J, Ayebare B, Nyombi A, Manyonge C, Patrick AJ, Fredrick K, and Joloba ML

Subjects

Humans, COVID-19 Testing methods, Uganda, Pilot Projects, COVID-19 diagnosis, SARS-CoV-2 isolation & purification, Specimen Handling methods, Specimen Handling standards, Laboratory Proficiency Testing, Developing Countries

Abstract

Introduction: When COVID-19 hit the world in 2019, an enhanced focus on diagnostic testing for SARS-CoV-2 was essential for a successful pandemic response. Testing laboratories stretched their capabilities for the new coronavirus by adopting different test methods. The necessity of having external quality assurance (EQA) mechanisms was even more critical due to this rapid expansion. However, there was a lack of experience in providing the necessary SARS-CoV-2 EQA materials, especially in locations with constrained resources., Objective: We aimed to create a PT (Proficiency testing) programme based on the Dried Tube Specimens (DTS) method that would be a practical option for molecular based SARS-CoV-2 EQA in Low- and Middle-Income Countries., Methods: Based on previous ISO/IEC 17043:2010 accreditation experiences and with assistance from the US Centers for Disease Control and Prevention, The Supranational Reference Laboratory of Uganda (adapted the DTS sample preparation method and completed a pilot EQA program between 2020 and 2021. Stability and panel validation testing was conducted on the designed materials before shipping to pilot participants in six African countries. Participants received a panel containing five SARS-CoV-2 DTS samples, transported at ambient conditions. Results submitted by participants were compared to validation results. Participants were graded as satisfactory (≥ 80%) or unsatisfactory (< 80%) and performance reports disseminated., Results: Our SARS-CoV-2 stability experiments showed that SARS-CoV-2 RNA was stable (-15 to -25 °C, 4 to 8 °C, (18 to 28 °C) room temperature and 35 to 38 °C) as well as DTS panels (4 to 8 °C, 18 to 28 °C, 35 to 38 °C and 45 °C) for a period of 4 weeks. The SARS-CoV-2 DTS panels were successfully piloted in 35 test sites from Zambia, Malawi, Mozambique, Nigeria, and Seychelles. The pilot results of the participants showed good accuracy, with an average of 86% (30/35) concordance with the original SARS CoV-2 expectations., Conclusion: The SARS-CoV-2 DTS PT panel is reliable, stable at ambient temperature, simple to prepare and requires minimal resources., (© 2024. The Author(s).)

Published

2024

40. Multinational proficiency tests for EGFR exon 20 insertions reveal that the assay design matters.

Author

Ihle MA, Heydt C, Schultheis AM, Stöhr R, Haller F, Herold S, Aust D, Dietmaier W, Evert M, Eszlinger M, Haak A, Laßmann S, Vorholt D, Breitenbücher F, Werner M, Streubel A, Mairinger T, Grassow-Narlik M, and Merkelbach-Bruse S

Subjects

Humans, Laboratory Proficiency Testing, Antibodies, Bispecific therapeutic use, Mutagenesis, Insertional, Protein Kinase Inhibitors therapeutic use, ErbB Receptors genetics, Exons, High-Throughput Nucleotide Sequencing methods, Carcinoma, Non-Small-Cell Lung genetics, Lung Neoplasms genetics

Abstract

Insertion mutations in exon 20 of the epidermal growth factor receptor gene (EGFR exon20ins) are rare, heterogeneous alterations observed in non-small cell lung cancer (NSCLC). With a few exceptions, they are associated with primary resistance to established EGFR tyrosine kinase inhibitors (TKIs). As patients carrying EGFR exon20ins may be eligible for treatment with novel therapeutics-the bispecific antibody amivantamab, the TKI mobocertinib, or potential future innovations-they need to be identified reliably in clinical practice for which quality-based routine genetic testing is crucial. Spearheaded by the German Quality Assurance Initiative Pathology two international proficiency tests were run, assessing the performance of 104 participating institutes detecting EGFR exon20ins in tissue and/or plasma samples. EGFR exon20ins were most reliably identified using next-generation sequencing (NGS). Interestingly, success rates of institutes using commercially available mutation-/allele-specific quantitative (q)PCR were below 30% for tissue samples and 0% for plasma samples. Most of these mutation-/allele-specific (q)PCR assays are not designed to detect the whole spectrum of EGFR exon20ins mutations leading to false negative results. These data suggest that NGS is a suitable method to detect EGFR exon20ins in various types of patient samples and is superior to the detection spectrum of commercially available assays., (© 2024. The Author(s).)

Published

2024

41. PCNEO, a New Proficiency Testing Program for Flow Cytometric Analysis of Plasma Cell Neoplasms From the College of American Pathologists Diagnostic Immunology and Flow Cytometry Committee.

Author

Dorfman DM, Devitt KA, Cui W, Bashleben C, Naharro ECF, Hedley B, Hupp M, Karlon WJ, Murphy CE, Cherian S, Olteanu H, Seifert RP, Rosado FN, and Linden MA

Subjects

Humans, United States, Societies, Medical, Multiple Myeloma diagnosis, Multiple Myeloma pathology, Multiple Myeloma immunology, Pathologists, Plasma Cells pathology, Plasma Cells immunology, Immunophenotyping methods, Pathology, Clinical standards, Pathology, Clinical methods, Flow Cytometry methods, Flow Cytometry standards, Laboratory Proficiency Testing, Neoplasms, Plasma Cell diagnosis

Abstract

Context.—: In 2018 the College of American Pathologists Diagnostic Immunology and Flow Cytometry Committee designed and implemented a new plasma cell neoplasia flow cytometry proficiency testing program-PCNEO-to allow clinical flow cytometry laboratories to monitor and assess their performance compared with a peer group., Objective.—: To report the results from the first 4 years of the PCNEO program., Design.—: Program participants were sent 2 sets of challenges per year, each including 1 wet challenge and 2 dry challenges, with associated clinical and laboratory findings. The wet challenges were composed of myeloma cell line specimens (with or without dilution in preserved whole blood) for flow cytometric analysis. The dry (paper) challenges were composed of clinical case summaries and images of flow cytometric test results from various flow cytometry laboratories of committee members., Results.—: A total of 116 to 145 laboratories from 17 countries enrolled in the proficiency testing program. For the wet challenges, almost all participants (97%-100%; cumulative, 98.2%) correctly identified the presence of neoplastic plasma cell populations based on flow cytometric analysis of undiluted myeloma cell lines. Slightly fewer participants (89.0%-97.4%; cumulative, 95.2%) correctly identified the presence of neoplastic plasma cell populations based on flow cytometric analysis of diluted myeloma cell lines (10% or 50% dilutions into peripheral blood) intended to better represent a typical clinical sample. There was generally agreement among 80% or more of participants for positive or negative staining for CD38, CD138, CD19, CD20, and surface and cytoplasmic κ and λ light chains. Similarly, 84% to 100% of participants were able to correctly identify the presence of neoplastic plasma cell populations in paper challenges, including the presence of small, neoplastic plasma cell populations (0.01%-5.0% clonal plasma cells) and the presence of nonneoplastic plasma cell populations (correctly identified by 91%-96% of participants)., Conclusions.—: Participant performance in the new proficiency testing program was excellent overall, with the vast majority of participants able to perform flow cytometric analysis and identify neoplastic plasma cell populations and to identify small plasma cell clones or expanded populations of reactive plasma cells in dry challenge flow cytometry results. This program will allow laboratories to verify the accuracy of their testing program and test interpretations for the assessment of patients suspected of having a plasma cell neoplasm., Competing Interests: All authors are current or past members of the College of American Pathologists Diagnostic Immunology and Flow Cytometry Committee, except for Bashleben, who is an employee of the College of American Pathologists., (© 2024 College of American Pathologists.)

Published

2024

42. Reporting and Establishment of Reference Intervals for Antiphospholipid Antibody Immunoassays: A Survey of Participants in the College of American Pathologists Proficiency Testing Program.

Author

Tebo AE, Willis R, Nwosu A, Bashleben C, Fox DA, Linden MA, and Karlon WJ

Subjects

Humans, Reference Values, Laboratory Proficiency Testing, United States, Immunoassay standards, Immunoassay methods, Immunoglobulin M blood, Immunoglobulin G blood, Surveys and Questionnaires, beta 2-Glycoprotein I immunology, Pathologists, Enzyme-Linked Immunosorbent Assay, Antibodies, Antiphospholipid blood, Antibodies, Antiphospholipid analysis, Antiphospholipid Syndrome diagnosis, Antiphospholipid Syndrome immunology, Antiphospholipid Syndrome blood

Abstract

Context.—: Misdiagnosis of antiphospholipid syndrome can occur owing to the wide diversity of antiphospholipid (aPL) assays and a lack of international calibrators and harmonized reference intervals., Objective.—: To assess laboratory practices regarding reporting and establishing reference intervals for immunoglobulin (Ig) G/IgM anti-cardiolipin (aCL) and anti-beta-2 glycoprotein I (anti-β2GPI) assays., Design.—: Supplemental questions related to reporting and establishing reference ranges for aPL assays were sent as part of the Antiphospholipid Antibody (ACL)-B 2019 College of American Pathologists (CAP) proficiency testing survey. The response rate and methods assessment details were determined, as well as qualitative and quantitative results for 3 test samples., Results.—: The number of participants reporting results for IgG aCL (n = 489), IgM aCL (n = 476), IgG anti-β2GPI (n = 354), and IgM anti-β2GPI (n = 331) varied by antibody type. The enzyme-linked immunosorbent assay (ELISA) (up to 58.6%, 260 of 444) was the most used method; others included multiplex (from 18.9% to 23.9%), fluorescence enzyme immunoassay (14.4%-17.6%), and chemiluminescence immunoassay (6.5%-9.0%). More respondents reported quantitative than qualitative results, and manufacturer cutoff ranges were used by 92.9% and 94.2% of respondents for aCL and anti-β2GPI, respectively. Despite variation in the use of semiquantitative ranges, qualitative negative/positive reporting of the test samples achieved almost 100% consensus. Qualitative consensus was met in contrast to the wide range of quantitative results obtained for each analyte across different kits., Conclusions.—: ELISA remains the most used method for detecting aPL antibodies, with most laboratories reporting quantitative results based on manufacturers' suggested reference ranges. The categorization of quantitative results as equivocal, weak positive, or positive for responders using kits from the same manufacturer was variable., Competing Interests: The authors have no relevant financial interest in the products or companies described in this article., (© 2024 College of American Pathologists.)

Published

2024

43. Significant Variability in the Identification and Reporting of Band Neutrophils by Participants Enrolled in the College of American Pathologists Proficiency Testing Program: Time for a Change.

Author

Vergara-Lluri M, Kovach AE, Nakashima MO, Bradley KT, Mahe E, Tsao L, Savage NM, Salansky SA, Long T, Perkins SL, Hsi ED, Pozdnyakova O, and Bhargava P

Subjects

Humans, Leukocyte Count, Surveys and Questionnaires, United States, Pathologists, Reproducibility of Results, Pathology, Clinical standards, Societies, Medical, Sepsis diagnosis, Observer Variation, Neutrophils cytology, Neutrophils pathology, Laboratory Proficiency Testing

Abstract

Context.—: Increased band neutrophils in blood smear differential counts ("bandemia") are entrenched in medicine as a flag for sepsis. However, laboratory hematology experts have long advocated for discontinuation of reporting bands separately from segmented neutrophils because of poor sensitivity and specificity, poor interobserver agreement, and availability of alternative biomarkers for sepsis., Objective.—: To describe band neutrophil reporting practices and reproducibility of band classification among laboratories participating in the College of American Pathologists (CAP) proficiency testing (PT) program., Design.—: A survey questionnaire was distributed to hematology PT participants. A subsequent morphologic challenge included 12 preselected cell identifications of segmented neutrophils, bands, and metamyelocytes, and a 100-cell manual differential count of a digitally scanned blood smear., Results.—: Among laboratories that reported manual differentials, most respondents reported bands (4554 of 5268; 86.4%). Only 3222 of 4412 respondents (73.0%) provided band reference ranges. Though participants classified "easy" band neutrophils well (78.0%-98.3%), categorization of cell identifications for "moderate" and "difficult" bands was poor (3.1%-39.0% of laboratories), with classification instead as segmented neutrophils. This pattern was seen regardless of laboratory demographic characteristics. Marked variability in band counts was observed on the 100-cell differential count for both CAP PT participants and CAP Hematology and Clinical Microscopy Committee (HCMC) members (coefficients of variation, 55.8% and 32.9%, respectively). Variability was significantly improved when segmented and band neutrophils were grouped together (coefficients of variation, 6.2% and 5.0%, respectively)., Conclusions.—: Most CAP PT-participating laboratories report band counts, many without reference ranges. The survey confirms significant interlaboratory variability of band enumeration when bands are separately identified from segmented neutrophils. This study reaffirms the CAP Hematology and Clinical Microscopy Committee's strong recommendation to group segmented and band neutrophils together in manual differential counts., Competing Interests: All authors are past or present members of the College of American Pathologists Hematology and Clinical Microscopy subcommittee., (© 2024 College of American Pathologists.)

Published

2024

44. Proficiency of phenotypic drug susceptibility testing for Mycobacterium tuberculosis in China, 2008-2021.

Author

Song Y, Zhao B, Wang S, Zheng Y, Zhou Y, Ou X, Xia H, and Zhao Y

Subjects

China, Humans, Laboratory Proficiency Testing, Reproducibility of Results, Phenotype, Amikacin pharmacology, Amikacin therapeutic use, Pyrazinamide therapeutic use, Mycobacterium tuberculosis drug effects, Microbial Sensitivity Tests, Antitubercular Agents pharmacology, Antitubercular Agents therapeutic use

Abstract

To analyze the results of proficiency testing for anti-tuberculosis drug susceptibility testing (DST) in China. Number of laboratory participating the proficiency testing performed DST, and the sensitivity, specificity, reproducibility, and accordance rate were calculated from data of 13 rounds proficiency testing results for DST from 2008 to 2021. A total of 30 and 20 strains of Mycobacterium tuberculosis with known susceptibility results were sent to each laboratory in 2008 to 2019, 2020 and 2021, respectively. The number of participating laboratories ranged from 30 in 2009 to 546 in 2021. L-J DST was the predominant method. The specificity presented relatively higher than sensitivity. Improvement of specificity were observed for all drugs through the years, while sensitivity did not show improvement for amikacin and capreomycin. Accordance rate of pyrazinamide and kanamycin and reproducibility of capreomycin and pyrazinamide were not significantly improved through the years. Most of the participating laboratories significantly improved the quality of their DST through the consecutive rounds of proficiency testing except for second-line injectable drugs and pyrazinamide. The results highlight the importance of developing novel and/or improving existing methods for phenotypic DST for certain drugs., Competing Interests: The authors have declared that no competing interests exist., (Copyright: © 2024 Song et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.)

Published

2024

45. Clarification of Information in "Navigating Next-Generation Sequencing Laboratory Developed Tests: A Critical Look at Proficiency Testing, US Food and Drug Administration Regulations, and Clinical Laboratory Performance Tests".

Author

Lockwood CM

Subjects

United States, Humans, Laboratories, Clinical, United States Food and Drug Administration, High-Throughput Nucleotide Sequencing, Laboratory Proficiency Testing

Abstract

Competing Interests: The author has no relevant financial interest in the products or companies described in this article.

Published

2024

46. RNA Sequencing for Solid Tumor Fusion Gene Detection: Proficiency Testing Practice and Performance Comparison.

Author

Bridge JA, Halling KC, Moncur JT, Souers RJ, Hameed MR, Fernandes H, Roy A, Surrey L, Tafe LJ, Vasalos P, and Lopez-Terrada DH

Subjects

Humans, Oncogene Proteins, Fusion genetics, Sequence Analysis, RNA, Neoplasms genetics, Neoplasms diagnosis, Gene Fusion, Sensitivity and Specificity, Laboratory Proficiency Testing, High-Throughput Nucleotide Sequencing

Abstract

Context: Next-generation sequencing-based approaches using RNA have increasingly been used by clinical laboratories for the detection of fusion genes, intragenic rearrangements, and exon-skipping events. Correspondingly, the College of American Pathologists (CAP) has advanced RNA sequencing proficiency testing (PT) to ensure optimal performance of these assays., Objective: To report on laboratory performance and practices of RNA sequencing for the detection of fusion genes, intragenic rearrangements, and exon-skipping events using CAP PT data from 8 mailings (2018-A through 2021-B)., Design: CAP PT RNA sequencing program results from 153 laboratories across 24 proficiency test specimens, interrogating 22 distinct engineered fusion transcripts, were analyzed for correct identification of the fusion event, associated performance variables, and laboratory practices., Results: Overall, the 4-year program detection rate (sensitivity) was 95.5% (1486 of 1556 results). False-negative rates were 3.6% (53 of 1463) and 18.3% (17 of 93) for fusion gene and intragenic rearrangement/exon-skipping events, respectively. Only 19 false-positive results were reported among the 8 PT mailings, and most were likely the result of preanalytical or postanalytical errors. There were no practice characteristics (eg, instrumentation, sequencing method) significantly associated with the fusion detection results., Conclusions: These data reveal a high overall sensitivity and specificity for fusion gene detection by participating laboratories using clinical RNA sequencing. Performance was comparable across all laboratories, regardless of methodology. The fraction of false-negative results for intragenic rearrangement/exon-skipping events was greater than that for the chimeric fusion genes. False-negative results could not be attributed to any specific practice characteristics., Competing Interests: The identification of specific products or scientific instrumentation is considered an integral part of the scientific endeavor and does not constitute endorsement or implied endorsement on the part of the author, Department of Defense (DoD), or any component agency. The views expressed in this article are those of the authors and do not reflect the official policy of the Department of Army/Navy/Air Force, DoD, or US government., (© 2024 College of American Pathologists.)

Published

2024

47. External quality assurance in the era of standardization.

Author

Theodorsson E, Meijer P, and Badrick T

Subjects

Laboratories, Quality Assurance, Health Care, Reference Standards, Clinical Laboratory Techniques, Laboratory Proficiency Testing

Abstract

Metrology in clinical chemistry aims to ensure the equivalence of measurement results from different in-vitro diagnostic measurement devices (IVD MD) for use in healthcare. The metrological traceability of measurement results to higher-order references is the cornerstone to achieving equivalent results. However, other fundamentals are also needed, including the commutability of reference materials and external quality assessment (EQA) materials for monitoring the equivalence of measurement results at the end-user level. This manuscript summarizes the findings and opinions expressed at the Joint Community for Traceability in Laboratory Medicine (JCTLM) workshop held on December 4-5, 2023. The workshop explored the relationship between EQA/proficiency testing and metrological traceability to higher-order references. EQA monitors the equivalence of measurement results from end-user IVD MDs. The workshop discussed the role and challenges of using EQA to improve and maintain the equivalence of measurement results. It also elucidated current developments in establishing the clinical suitability of laboratory results expressed as analytical performance specifications (APS)., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 The Author(s). Published by Elsevier B.V. All rights reserved.)

Published

2024

48. Top-down and bottom-up approaches for the estimation of measurement uncertainty in coagulation assays.

Author

Lim, Yong Kwan, Kweon, Oh Joo, Lee, Mi-Kyung, Kim, Bohyun, and Kim, Hye Ryoun

Subjects

*BLOOD coagulation, *PARTIAL thromboplastin time, *INTERNATIONAL normalized ratio, *PROTEIN C

Abstract

Background: The assessment of measurement uncertainty (MU) in clinical laboratories is essential to the reliable interpretation of results in clinical laboratories. However, despite the introduction of various methods for the expression of uncertainty in measurement, the MUs of coagulation tests have not been extensively studied. The aim of this study was to quantify the MU of various coagulation assays according to international guidelines and to report an expected confidence in the quality of coagulation assays. Methods: We selected activated partial thromboplastin time, international normalized ratio (INR), protein C/S, antithrombin, fibrinogen, and Factor V/VIII/X to quantify the MUs of two coagulation testing systems: ACL TOP 750 CTS (Instrumentation Laboratory, Bedford, MA, USA) and STA Compact (Diagnostica Stago, Asnières-sur-Seine, France). We used international standards and interlaboratory comparison results in accordance with international guidelines in a top-down approach to the assessment of MU. For INR, MU was estimated in a bottom-up approach using reference thromboplastin and certified plasmas. Results: Top-down approaches resulted in MUs between 3.3% and 21.3% for each measurand. In the bottom-up approach, MUs of INR values ranged from 10.9% to 26.4% and showed an upward trend as INR increased. Conclusions: In this study, we were successful in quantifying MU of coagulation assays using practical methods. Our results demonstrated that top-down and bottom-up approaches were adequate for coagulation assays. However, some assays showed significant biases against international standards; therefore, standardization would be necessary to ensure more reliable patient results. [ABSTRACT FROM AUTHOR]

Published

2020

49. Retrospection of Anti-Blood Group Antibody Proficiency Testing Data Using the Geometric Mean and Standard Deviation.

Author

Yang, John Jeongseok, Chung, Yousun, Kim, Hyungsuk, Ko, Dae-Hyun, Hwang, Sang-Hyun, and Oh, Heung-Bum

Subjects

*STANDARD deviations, *ABILITY, *IMMUNOGLOBULINS, *ARITHMETIC mean, *STATISTICS, *BLOOD group incompatibility, *BLOOD groups, *MEDICAL laboratories, *QUALITY assurance, *RETROSPECTIVE studies

Abstract

Objectives: We reanalyzed the data from proficiency testing (PT) to assess the effect of the geometric mean in the statistical analysis of immunohematologic data.Methods: Using the five most recent anti-blood group antibody titer participant summary results, the geometric mean (GM) ±2 × geometric standard deviation (GSD) was used as the comparative consensus criterion to mode ±2 titers.Results: Using the PT evaluation criterion of mode ±2 titers, the mean percentages of participants with acceptable results were 97.5% and 97.8% for anti-A and anti-D, respectively. When applying GM ±2 GSD, the mean percentages of acceptable results were 96.1% (anti-A) and 96.1% (anti-D). The percentages of responses included in each consensus criterion were lower using GM ±2 GSD, with a few exceptions.Conclusions: Geometric means are more robust and precise in visualizing the central tendency. This method can improve the statistical robustness of PT evaluations. [ABSTRACT FROM AUTHOR]

Published

2020

50. Differences between Educational and Regulatory External Quality Assurance/Proficiency Testing Schemes

Author

Tony, Badrick, Graham, Jones, W Greg, Miller, Mauro, Panteghini, Andrew, Quintenz, Sverre, Sandberg, and Michael, Spannagl

Subjects

Laboratory Proficiency Testing, Quality Assurance, Health Care, Biochemistry (medical), Clinical Biochemistry, Humans, Laboratories, Settore BIO/12 - Biochimica Clinica e Biologia Molecolare Clinica

Published

2022