Your search keyword '"Rongxue Peng"' showing total 33 results

1. Interlaboratory variability of HER2 fluorescence in situ hybridization testing in breast cancer: results of a multicenter proficiency-testing ring study in China

Author

Rongxue Peng, Kuo Zhang, Guigao Lin, and Jinming Li

Subjects

Breast cancer, HER2, FISH, Standardization, Quality assurance, Pathology, RB1-214

Abstract

Abstract Background Accurate detection of human epidermal growth factor receptor 2 (HER2) gene amplification via fluorescence in situ hybridization (FISH) is necessary to determine HER2 status. Although many attempts have been made to increase the consistency of the results, the actual situation still needs to be determined. To investigate the latest interlaboratory variability of HER2 FISH testing for breast cancer, a multicenter proficiency-testing ring study was conducted in China. Methods A total of ten samples, each exhibiting distinct HER2 signal patterns and genetic heterogeneity, were distributed to 169 laboratories for HER2 FISH analysis. Data comprising both the results of the tests and feedback from questionnaires were compiled for comprehensive evaluation. Results The overall agreement among the participating laboratories was substantial to almost perfect, with a Fleiss’ kappa value of 0.765–0.911. However, it is important to note that cases with characteristics of HER2 signals near the critical cutoff range or with genetic heterogeneity showed lower congruence, poorer reproducibility, and higher variability (Fleiss’ kappa: 0.582). Our questionnaire showed that 52.2% (86/168) of the participants did not perform validation after their operation procedures or interpretation criteria were updated, and 75.6% (121/160) of the participants did not establish standard interpretation procedures. Since these laboratories showed worse performance (P

Published

2024

2. A novel method for the preparation of reproducible, stable, and non-infectious quality control materials for Chlamydia trachomatis nucleic acid detection

Author

Jing Li, Kuo Zhang, Yanxi Han, Rongxue Peng, Lin Li, Jinming Li, and Guigao Lin

Subjects

cell lines, Chlamydia trachomatis, CRISPR/Cas9, nucleic acid amplification test, quality control, Microbiology, QR1-502

Abstract

ABSTRACT Chlamydia trachomatis (CT) is a significant sexually transmitted pathogen known to evoke severe complications, including infertility. Nucleic acid amplification tests (NAATs) are recommended by the World Health Organization to detect CT infection. Furthermore, the establishment of methods, performance validation, internal quality control, and external quality assessment for CT NAATs necessitate the utilization of quality control materials (QCs). QCs are specimens or solutions that are analyzed for quality control purposes in a test system. In this study, we established a novel cell line that stably integrates CT amplification target sequences for producing QCs for CT NAATs. Utilizing clustered regularly interspaced short palindromic repeats/CRISPR-associated protein 9 technology, we integrated the CT plasmid-mediated sequence (comprising the full length of the cryptic plasmid and the major outer membrane protein gene, 9,136 bp) into the MUC4 gene of HEK293T cells. Positive clones were screened through flow cytometric sorting, single-cell culture, and PCR-based identification, followed by the establishment of stable cell lines. These cells were then processed using optimized cell preservation procedures to prepare QCs. The sequence insertion copy number was confirmed by real-time quantitative PCR. This novel CT QCs demonstrate excellent clinical applicability, non-infectiousness, quantifiability, and stability. With an integrated sequence exceeding 9 kb in length, it offers exceptional flexibility for adapting to new kit developments. Furthermore, maintaining a well-defined copy number and stable shelf life, the QCs closely aligns with the quality control requirements of CT NAATs. This study presents an innovative method for preparing QCs for CT nucleic acid detection, making a valuable contribution to improving the performance of CT NAATs.IMPORTANCEUntreated CT infections impose significant burdens on individuals and communities, underscoring the importance of early and accurate testing via CT NAATs for disease control. QCs are instrumental in identifying testing process issues. Hence, we developed a cell line integrating CT-amplified target sequences as readily accessible non-infectious QCs. These QCs boast several advantages: the integration of over 9 kb of CT sequence allows for broad applicability, allowing flexible adaptation to the development of new kits. Confirming the CT sequence copy number provides a reliable basis for QC concentration preparation and kit detection limit evaluation. Optimized preservation protocol enhances QC stability during storage, facilitating convenient shipment to clinical laboratories at ambient temperatures. In summary, our novel CT QCs offer a powerful tool for improving CT NAAT performance and present a fresh perspective on QC preparation for detecting nucleic acids from intracellular parasitic pathogens.

Published

2024

3. Enhancing the quality of panel-based tumor mutation burden assessment: a comprehensive study of real-world and in-silico outcomes

Author

Yuanfeng Zhang, Duo Wang, Zihong Zhao, Rongxue Peng, Yanxi Han, Jinming Li, and Rui Zhang

Subjects

Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

Abstract Targeted panel-based tumor mutation burden (TMB) assays are widely employed to guide immunotherapy for patients with solid tumors. However, the accuracy and consistency of this method can be compromised due to the variability in technical details across different laboratories, particularly in terms of panel size, somatic mutation detection and TMB calculation rules. Currently, systematic evaluations of the impact of these technical factors on existing assays and best practice recommendations remain lacking. We assessed the performance of 50 participating panel-based TMB assays involving 38 unique methods using cell line samples. In silico experiments utilizing TCGA MC3 datasets were performed to further dissect the impact of technical factors. Here we show that the panel sizes beyond 1.04 Mb and 389 genes are necessary for the basic discrete accuracy, as determined by over 40,000 synthetic panels. The somatic mutation detection should maintain a reciprocal gap of recall and precision less than 0.179 for reliable psTMB calculation results. The inclusion of synonymous, nonsense and hotspot mutations could enhance the accuracy of panel-based TMB assay. A 5% variant allele frequency cut-off is suitable for TMB assays using tumor samples with at least 20% tumor purity. In conclusion, this multicenter study elucidates the major technical factors as sources of variability in panel-based TMB assays and proposed comprehensive recommendations for the enhancement of accuracy and consistency. These findings will assist clinical laboratories in optimizing the methodological details through bioinformatic experiments to enhance the reliability of panel-based methods.

Published

2024

4. Quartet DNA reference materials and datasets for comprehensively evaluating germline variant calling performance

Author

Luyao Ren, Xiaoke Duan, Lianhua Dong, Rui Zhang, Jingcheng Yang, Yuechen Gao, Rongxue Peng, Wanwan Hou, Yaqing Liu, Jingjing Li, Ying Yu, Naixin Zhang, Jun Shang, Fan Liang, Depeng Wang, Hui Chen, Lele Sun, Lingtong Hao, The Quartet Project Team, Andreas Scherer, Jessica Nordlund, Wenming Xiao, Joshua Xu, Weida Tong, Xin Hu, Peng Jia, Kai Ye, Jinming Li, Li Jin, Huixiao Hong, Jing Wang, Shaohua Fan, Xiang Fang, Yuanting Zheng, and Leming Shi

Subjects

Biology (General), QH301-705.5, Genetics, QH426-470

Abstract

Abstract Background Genomic DNA reference materials are widely recognized as essential for ensuring data quality in omics research. However, relying solely on reference datasets to evaluate the accuracy of variant calling results is incomplete, as they are limited to benchmark regions. Therefore, it is important to develop DNA reference materials that enable the assessment of variant detection performance across the entire genome. Results We established a DNA reference material suite from four immortalized cell lines derived from a family of parents and monozygotic twins. Comprehensive reference datasets of 4.2 million small variants and 15,000 structural variants were integrated and certified for evaluating the reliability of germline variant calls inside the benchmark regions. Importantly, the genetic built-in-truth of the Quartet family design enables estimation of the precision of variant calls outside the benchmark regions. Using the Quartet reference materials along with study samples, batch effects are objectively monitored and alleviated by training a machine learning model with the Quartet reference datasets to remove potential artifact calls. Moreover, the matched RNA and protein reference materials and datasets from the Quartet project enables cross-omics validation of variant calls from multiomics data. Conclusions The Quartet DNA reference materials and reference datasets provide a unique resource for objectively assessing the quality of germline variant calls throughout the whole-genome regions and improving the reliability of large-scale genomic profiling.

Published

2023

5. Development of a Novel Reference Material for Tumor Mutational Burden Measurement Based on CRISPR/Cas9 Technology

Author

Rongxue Peng, Guigao Lin, Lin Li, and Jinming Li

Subjects

CRISPR/Cas9, tumor mutational burden, next-generation sequencing, reference material, standardization, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

As a biomarker that affects treatment decisions of immune checkpoint inhibitors, the accuracy, reliability, and comparability of tumor mutational burden (TMB) estimation is of paramount importance. To improve the consistency and reliability of these tests, qualified reference materials providing ground-truth data are crucial. In this study, we developed a set of formalin-fixed and paraffin-embedded (FFPE) samples with different TMB values as the novel reference materials for TMB estimation. By introducing several clinically relevant variants in MutS Homolog 2 (MSH2) gene and DNA polymerase epsilon (POLE) gene into human cell lines using CRISPR/Cas9 technology, we first constructed four typical cell lines which verified with hypermutator or ultramutator phenotype. Followed by cell mixing and paraffin embedding, the novel FFPE samples were prepared. It was confirmed that our novel FFPE samples have sufficient quantity of cells, high reproducibility, and they can provide matched wild type sample as the genetic background. The double-platform whole exome sequencing validation showed that our FFPE samples were also highly flexible as they containing different TMB values spanning a clinically relevant range (2.0–106.1 mut/Mb). Without limitations on production and TMB values, our novel FFPE samples based on CRISPR/Cas9 editing are suitable as candidate reference materials. From a practical point of view, these samples can be used for the validation, verification, internal quality control, and proficiency testing of TMB assessment.

Published

2022

6. Adaptation of ACMG-ClinGen Technical Standards for Copy Number Variant Interpretation Concordance

Author

Kuo Zhang, Guigao Lin, Dongsheng Han, Yanxi Han, Rongxue Peng, and Jinming Li

Subjects

copy number variant, classification and interpretation, concordance, ACMG-ClinGen technical standards, inter-laboratory, Genetics, QH426-470

Abstract

This study aimed to evaluate inter-laboratory classification concordance for copy number variants (CNVs) with a semiquantitative point-based scoring metric recommended by the American College of Medical Genetics and Genomics (ACMG) and Clinical Genome Resources (ClinGen). A total of 234 CNVs distributed by the National Center of Clinical Laboratories (NCCLs), and 72 CNVs submitted by different laboratories, were distributed to nine clinical laboratories performing routine clinical CNV testing in China and independently classified across laboratories. The overall inter-laboratory complete classification concordance rate of the 234 distributed CNVs increased from 18% (41/234) to 76% (177/234) using the scoring metric compared to the laboratory's previous method. The overall inter-laboratory complete classification concordance rate of the 72 submitted CNVs was 65% (47/72) using the scoring metrics. The 82 variants that initially did not reach complete concordance classification and 1 additional CNV deletion were reviewed; 34 reached complete agreement, and the overall post-review complete concordance rate was 85% (260/306). Additionally, the overall percentage of classification discordance possibly impacting medical management [i.e., pathogenic (P) or likely pathogenic (LP) vs. variant of uncertain significance (VUS)] was 11% (35/306). The causes of initial and final discordance in the classification were identified. The ACMG-ClinGen framework has promoted consistency in interpreting the clinical significance of CNVs. Continuous training among laboratories, further criteria and additional clarification of the standards, sharing classifications and supporting evidence through public database, and ongoing work for dosage sensitive genes/regions curation will be beneficial for harmonization of CNVs classification.

Published

2022

7. Accuracy of analysis of cfDNA for detection of single nucleotide variants and copy number variants in breast cancer

Author

Xin Yang, Kuo Zhang, Caiji Zhang, Rongxue Peng, and Chengming Sun

Subjects

PIK3CA, TP53, ESR1, cfDNA, Mutation, Breast cancer, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

Abstract Background Gene variants are dependable and sensitive biomarkers for target-specific therapies in breast cancer (BC). However, detection of mutations within tissues has many limitations. Plasma circulating free DNA (cfDNA) has been reported in many studies as an alternative tool for detection of mutations. But the diagnostic accuracy of cfDNA for most mutations in BC needs to be reviewed. This study was designed to perform comparative assessment of the diagnostic performance of cfDNA and DNA extracted from tissues for detection of single nucleotide variants (SNV) and copy number variants (CNV). Methods True-positive (TP), false-positive (FP), false-negative (FN), and true-negative (TN) values were extracted from each selected study. Pooled sensitivity, specificity, positive likelihood ratio (PLR), negative likelihood ratio (NLR), and diagnostic odds ratio (DOR) were calculated. Subgroup analysis and single study omitted analysis were performed to quantify and explain the study heterogeneity. Results Twenty eligible studies that involved 1055 cases were included in this meta-analysis. SNV studies in early breast cancer (EBC) subgroup are not suitable for meta-analysis owing to high heterogeneity. However, in advanced breast cancer (ABC) subgroup, the pooled sensitivity and specificity of detection of SNVs were 0.78 (0.71–0.84) and 0.92 (0.87–0.95), respectively. The summary receiver operative curve (SROC) exhibited an area under the curve (AUC) of 0.91(0.88–0.93). The pooled results of studies involving subgroups of PIK3CA, TP53, and ESR1 indicate that the diagnostic value of different genes is different, such as AUC for PIK3CA and TP53 were reported to be 0.96 (0.94–0.98) and 0.94 (0.91–0.95), respectively, and ESR1 had the lowest diagnostic value of 0.80 (0.76–0.83). Owing to the low sensitivity and AUC in the cases of CNV, there is no value for cfDNA-based detection of CNV based on insufficient amount of CNV data. Conclusion This meta-analysis suggests that the detection of gene mutations in cfDNA have adequate diagnostic accuracy and can be used as an alternative to the tumor tissue for detection of SNV but not for CNV in BC yet.

Published

2019

8. Correction: External Quality Assessment of Molecular Detection of Ebola Virus in China.

Author

Guojing Wang, Yu Sun, Kuo Zhang, Tingting Jia, Mingju Hao, Dong Zhang, Le Chang, Lei Zhang, Rui Zhang, Guigao Lin, Rongxue Peng, and Jinming Li

Subjects

Medicine, Science

Published

2016

9. External Quality Assessment of Molecular Detection of Ebola Virus in China.

Author

Guojing Wang, Yu Sun, Kuo Zhang, Tingting Jia, Mingju Hao, Dong Zhang, Le Chang, Lei Zhang, Rui Zhang, Guigao Lin, Rongxue Peng, and Jinming Li

Subjects

Medicine, Science

Abstract

In 2014, Ebola hemorrhagic fever broke out in West Africa. As contact between China and West Africa is frequent, the possibility that Ebola virus would enter China was high. Thus, an external assessment of the quality of Ebola virus detection was organized by the National Center for Clinical Laboratories in China. Virus-like particles encapsulating known sequences of epidemic strains of Ebola virus from 2014 were prepared as positive quality controls. The sample panel, which was composed of seven positive and three negative samples, was dispatched to 19 laboratories participating in this assessment of Ebola virus detection. Accurate detection was reported at 14 of the 19 participating laboratories, with a sensitivity of 91.43% and a specificity of 100%. Four participants (21.05%) reported false-negative results and were classified as "acceptable." One participant (5.26%) did not detect any positive samples and was thus classified as "improvable." Based on the results returned, the ability to detect weakly positive Ebola specimens should be improved. Furthermore, commercial assays and the standard primers offered by the Chinese Centers for Disease Control and Prevention were found to be most accurate and dependable for Ebola detection. A two-target detection approach is recommended for Ebola screening; this approach could reduce the probability of false-negative results. Additionally, standardization of operations and punctual adjustment of instruments are necessary for the control and prevention of Ebola virus.

Published

2015

10. Analysis of Clinical Laboratory Detecting Challenging Variants from Exome Sequencing Using Simulated Patient–Parent Trio Sample

Author

Kuo Zhang, Guigao Lin, Yanxi Han, Rongxue Peng, and Jinming Li

Subjects

Molecular Medicine, Pathology and Forensic Medicine

Published

2023

11. Reprogramming of Human B Cells from Secreting IgG to IgM by Genome Editing

Author

Guigao Lin, Kuo Zhang, Yanxi Han, Rongxue Peng, Jiawei Zhang, Dandan Li, and Jinming Li

Subjects

Gene Editing, Immunoglobulin M, Immunoglobulin G, Genetics, Humans, CRISPR-Cas Systems, Immunoglobulin E, RNA, Guide, Kinetoplastida, Immunoglobulin A, Biotechnology

Abstract

B lymphocytes are activated and regulated by their interactions with T cells, a process that results in one-way class switching of immunoglobulins (ig) from IgM to IgG, IgE, or IgA. In this study, we show the application of clustered regularly interspaced short palindromic repeat-Cas9-induced nonhomologous end joining in B cells to achieve reverse-directional Ig class switching. By electroporating Cas9 and guide RNA and a Cμ encoding donor into cells, we engineered IgG-secreting human B cell lines to switch to express IgM antibody. This approach offers a new potential path for the production of IgM antibodies.

Published

2022

12. Continual Improvement of the Reliability of Next-Generation Sequencing-Based ctDNA Analysis: A Long-Term Comparison of ctDNA Detection in China

Author

Rongxue, Peng, Rui, Zhang, and Jinming, Li

Subjects

Laboratory Proficiency Testing, Mutation, Biochemistry (medical), Clinical Biochemistry, Biomarkers, Tumor, High-Throughput Nucleotide Sequencing, Humans, Reproducibility of Results, Circulating Tumor DNA

Abstract

Background Since circulating tumor DNA (ctDNA) sequencing is increasingly being applied in clinical management of patients with cancer, its testing accuracy has become a matter of serious concern. To address this issue, a long-term ctDNA analysis proficiency testing (PT) scheme for next-generation sequencing (NGS) was launched in China in 2018, serving as an educational tool for assessing and improving the testing quality of NGS-based ctDNA detection. Methods Feedback from participating laboratories across 23 different PT samples containing different variants with varying variant allele frequency was collected between 2018 and 2021. To further show the landscape of changing conditions in accuracy and reliability of NGS-based ctDNA testing, performance was analyzed by evaluating the cfDNA extraction kits, testing panels, target enrichment strategies, and sequencing platforms. Results During the 4 years, 2745 results reported from 504 laboratories were evaluated. Only 66.3% of results from laboratories were entirely in concordance with the expected results. Nonetheless, along with an increasing number of participating laboratories, the number of errors occurring in laboratories, and the proportion of laboratories that experienced errors both showed a significant downward trend. No obvious differences in the error rates were found regarding the kit manufacturers or sequencing platform. Moreover, the individual performances of the laboratories improved when they participated in more PT scheme rounds. Conclusions These data demonstrated that the performance of individual Chinese laboratories for NGS-based ctDNA analysis continuously improved over time with participation in PT schemes. However, further care must also be taken in standardized operations and validations.

Published

2022

13. Delivery of microRNA-21-sponge and pre-microRNA-122 by MS2 virus-like particles to therapeutically target hepatocellular carcinoma cells

Author

Rongxue Peng, Jiawei Zhang, Rui Zhang, Jinming Li, and Dandan Li

Subjects

Carcinoma, Hepatocellular, Apoptosis, Peptide, General Biochemistry, Genetics and Molecular Biology, Virus, Downregulation and upregulation, Cell Movement, Cell Line, Tumor, microRNA, medicine, Humans, Original Research, Cell Proliferation, Levivirus, chemistry.chemical_classification, Messenger RNA, Expression vector, Liver Neoplasms, Gene Transfer Techniques, Genetic Therapy, Hep G2 Cells, medicine.disease, MicroRNAs, chemistry, Hepatocellular carcinoma, Cancer research, Artificial Virus-Like Particles

Abstract

MicroRNAs are related to the development of hepatocellular carcinoma and can serve as potential therapeutic targets. Therapeutic strategies increasing tumor-suppressive microRNAs and reducing oncogenic microRNAs have been developed. Herein, the effects of simultaneously altering two microRNAs using MS2 virus-like particles were studied. The sequences of microRNA-21-sponge and pre-microRNA-122 were connected and cloned into a virus-like particle expression vector. Virus-like particles containing microRNA-21-sponge and pre-microRNA-122 sequences were prepared and crosslinked with a cell-specific peptide targeting hepatocellular carcinoma cells. Delivery effects were studied using RT-qPCR and functional assays to investigate the level of target mRNAs, cell toxicity, and the effects of proliferation, invasion, and migration. Virus-like particles delivered miR-21-sponge into cells, with the Ct value reaching 10 at most. The linked pre-miR-122 was processed into mature miR-122. The mRNA targets of miR-21 were derepressed as predicted and upregulated 1.2–2.8-fold, and the expression of proteins was elevated correspondingly. Proliferation, migration, and invasion of HCC cells were inhibited by miR-21-sponge. Simultaneous delivery of miR-21-sponge and miR-122 further decreased proliferation, migration, and invasion by up to 34%, 63%, and 65%, respectively. And the combination promoted the apoptosis of HCC cells. In conclusion, delivering miR-21-sponge and miR-122 using virus-like particles modified by cell-specific peptides is an effective and convenient strategy to correct microRNA dysregulation in hepatocellular carcinoma cells and is a promising therapeutic strategy for hepatocellular carcinoma.

Published

2021

14. Continual Improvement of the Reliability of EML4-ALK Rearrangement Detection in Non–Small-Cell Lung Cancer

Author

Jiehong Xie, Rui Zhang, Jinming Li, Ping Tan, Yanxi Han, Guigao Lin, Rongxue Peng, Kuo Zhang, and Jiawei Zhang

Subjects

0301 basic medicine, Computer science, medicine.disease, Pathology and Forensic Medicine, Term (time), Reliability engineering, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, hemic and lymphatic diseases, 030220 oncology & carcinogenesis, medicine, Proficiency testing, Molecular Medicine, Anaplastic lymphoma kinase, Non small cell, ALK Rearrangement, Lung cancer, Reliability (statistics)

Abstract

The results of EML4-ALK testing are critical to manage ALK tyrosine kinase receptor inhibitor treatment. Thus, the accurate detection of ALK rearrangement is increasingly becoming a matter of serious concern. To address this issue, a long-term EML4-ALK proficiency testing (PT) scheme was launched in China in 2015, serving as an educational tool for assessing and improving the testing quality of EML4-ALK fusion detection. Responses across 20 different PT samples interrogating three different variants and wild-type samples were collected between 2015 and 2019. Performance was analyzed by evaluating the detection methods, kits, and pre-analytic practices used to further display the landscape of changing conditions of the reliability of EML4-ALK testing. During the 5 years, 3224 results reported from 988 laboratories were evaluated, with an overall error rate of 5.36%. Along with an increasing number of participating laboratories, the error rate within each of the different methods showed a significantly downward trend over the years. No obvious differences in the error rates were found regarding the testing methods or kit manufacturers. Moreover, the individual performance of the laboratories improved when they participated in more PT scheme rounds. The data demonstrated that the performance of individual Chinese laboratories for EML4-ALK testing continuously improved over time by participating PT schemes, regardless of their method. However, care must be taken in standardized operations and validations.

Published

2020

15. From Somatic Variants Toward Precision Oncology: An Investigation of Reporting Practice for Next-Generation Sequencing-Based Circulating Tumor DNA Analysis

Author

Jinming Li, Kwang Hong Tay, Tony Badrick, Nalishia Pillay, Martin Horan, Li Zhou, Rui Zhang, Rongxue Peng, and Sze Yee Chai

Subjects

0301 basic medicine, Cancer Research, medicine.medical_specialty, Cancer Diagnostics and Molecular Pathology, medicine.diagnostic_test, Standardization, business.industry, Concordance, DNA sequencing, Drug access, 03 medical and health sciences, Identification (information), 030104 developmental biology, 0302 clinical medicine, Oncology, Precision oncology, Circulating tumor DNA, 030220 oncology & carcinogenesis, medicine, Medical physics, business, Genetic testing

Abstract

BACKGROUND: With the accelerated development of next‐generation sequencing (NGS), identified variants, and targeted therapies, clinicians who confront the complicated and multifarious genetic information may not effectively incorporate NGS‐based circulating tumor DNA (ctDNA) analysis into routine patient care. Consequently, standardized ctDNA testing reports are of vital importance. In an effort to guarantee high‐quality reporting performance, we conducted an investigation of the current detection and reporting practices for NGS‐based ctDNA analysis. MATERIALS AND METHODS: A set of simulated ctDNA samples with known variants at known allelic frequencies and a corresponding case scenario were distributed to 66 genetic testing laboratories for ctDNA analysis. Written reports were collected to evaluate the detection accuracy, reporting integrity, and information sufficiency using 21 predefined criteria. RESULTS: Current reporting practices for NGS‐based ctDNA analysis were found to be far from satisfactory, especially regarding testing interpretation and methodological details. Only 42.4% of laboratories reported the results in complete concordance with the expected results. Moreover, 74.2% of reports only listed aberrations with direct and well‐known treatment consequences for the tumor type in question. Genetic aberrations for which experimental agents and/or drug access programs are available may thus be overlooked. Furthermore, methodological details for the interpretation of results were missing from the majority of reports (87.9%). CONCLUSION: This proof‐of‐principle study suggests that the capacity for accurate identification of variants, rational interpretation of genotypes, comprehensive recommendation of potential medications, and detailed description of methodologies need to be further improved before ctDNA analysis can be formally implemented in the clinic. IMPLICATIONS FOR PRACTICE: Accurate, comprehensive, and standardized clinical sequencing reports can help to translate complex genetic information into patient‐centered clinical decisions, thereby shepherding precision oncology into daily practice. However, standards, guidelines, and quality requirements for clinical reports of next‐generation sequencing (NGS)‐based circulating tumor DNA (ctDNA) analysis are currently absent. By using a set of simulated clinical ctDNA samples and a corresponding case scenario, current practices were evaluated to identify deficiencies in clinical sequencing reports of ctDNA analysis. The recommendations provided here may serve as a roadmap for the improved implementation of NGS‐based ctDNA analysis in the clinic.

Published

2019

16. External Quality Assessment for Molecular Detection of Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) in Clinical Laboratories

Author

Rui Zhang, Zhe Wang, Jing Yang, Shaohua Zhan, Rui Li, Jinming Li, Rongxue Peng, Jiping Shi, Runling Zhang, Yuqing Chen, and Yanxi Han

Subjects

0301 basic medicine, Viral nucleic acid, biology, business.industry, viruses, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Nucleic acid amplification technique, Gold standard (test), biology.organism_classification, Virology, Pathology and Forensic Medicine, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, Real-time polymerase chain reaction, 030220 oncology & carcinogenesis, Bacteriophage MS2, External quality assessment, Medicine, Molecular Medicine, Viral rna, business

Abstract

Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) poses a huge threat to public health. Viral nucleic acid testing is the diagnostic gold standard and can play an important role in the prevention and control of this infection. In this study, bacteriophage MS2 virus-like particles encapsulating specific RNA sequences of SARS-CoV-2 and other coronaviruses were prepared by genetic engineering. The assessment panel, consisting of four positive samples with concentrations of 2.8, 3.5, 4.2, and 4.9 log10 copies/mL and five negative samples with other human coronaviruses, was prepared and distributed to evaluate the accuracy of routine viral RNA detection. Results of 931 panels from 844 laboratories were collected. The overall percentage agreement, positive percentage agreement (PPA), and negative percentage agreement, defined as the percentage of agreement between the correct results and total results submitted for all, positive, and negative samples were 96.8% (8109/8379), 93.9% (3497/3724), and 99.1% (4612/4655), respectively. For samples with concentrations of 4.9 and 4.2 log10 copies/mL, the PPAs were >95%. However, for 3.5 and 2.8 log10 copies/mL, the PPAs were 94.6% (881/931) and 84.9% (790/931), respectively. For all negative samples, the negative percentage agreement values were >95%. Thus, most laboratories can reliably detect SARS-CoV-2. However, further improvement and optimization are required to ensure the accuracy of detection in panel members with lower concentrations of viral RNA.

Published

2021

17. Utilizing CRISPR/Cas9 technology to prepare lymphoblastoid cell lines harboring genetic mutations for generating quality control materials in genetic testing

Author

Runling Zhang, Jiawei Zhang, Peng Gao, Rui Zhang, Rongxue Peng, Kun Chen, Rui Li, Jinming Li, and Li Zhou

Subjects

0301 basic medicine, Clinical Biochemistry, medicine.disease_cause, law.invention, 0302 clinical medicine, law, CRISPR-Associated Protein 9, Immunology and Allergy, CRISPR, Polymerase chain reaction, Research Articles, Sanger sequencing, Gene Editing, Mutation, stably Cas9 expressing cell line, medicine.diagnostic_test, Electroporation, in vitro transcribed gRNAs, quality control material, High-Throughput Nucleotide Sequencing, Hematology, Medical Laboratory Technology, lymphoblastoid cell line, 030220 oncology & carcinogenesis, symbols, Research Article, RNA, Guide, Kinetoplastida, Microbiology (medical), Quality Control, Computational biology, Biology, Transfection, genetic testing, Cell Line, 03 medical and health sciences, symbols.namesake, alpha-Thalassemia, medicine, Humans, Indel, CRISPR/Cas9, Genetic testing, Whole Genome Sequencing, Cas9, Biochemistry (medical), Public Health, Environmental and Occupational Health, 030104 developmental biology, CRISPR-Cas Systems

Abstract

Background To meet the requirements of the rapidly progressing genetic testing technologies in clinical laboratories, assuring the quality of genetic tests by utilizing appropriate quality control materials is of paramount importance. The CRISPR/Cas9 technology was used to prepare quality control materials because genome‐edited human cell lines are one of the major resources for quality control materials. Methods In this study, in vitro transcribed sgRNA were transfected into a Cas9‐expressing lymphoblastoid cell line (LCL)—by electroporation—to simulate the SEA‐type deletion observed in α‐thalassemia. The edited positive cell line was screened and identified by polymerase chain reaction (PCR) followed by Sanger sequencing. The whole‐genome sequencing was also performed to show evidence of predicted mutation. Results The results showed that electroporation of the in vitro transcribed gRNAs into stable Cas9‐expressing LCL was a more efficient gene‐editing technique as compared to plasmid‐mediated transfection, and that the positive rates could reach up to 35.9%. The predominance of indel sizes relative to the predicted deletion length was clustered between 10 and 0 bp. The results of whole‐genome sequencing also demonstrated the existence of SEA‐type deletion of α‐thalassemia. Conclusions Gene‐editing based on Cas9‐expressing LCL by electroporation of sgRNA was a more efficient approach to introduce mutations for generating quality control materials for genetic testing. The edited lymphoblastoid cell lines were feasible to serve as quality control materials in genetic testing.

Published

2020

18. The applications of CRISPR/Cas system in molecular detection

Author

Rongxue Peng, Li Zhou, Rui Zhang, and Jinming Li

Subjects

0301 basic medicine, Computer science, Reviews, single nucleotide variants, Review, Computational biology, medicine.disease_cause, Polymorphism, Single Nucleotide, DNA sequencing, 03 medical and health sciences, chemistry.chemical_compound, diagnostics, medicine, CRISPR, Guide RNA, Bacteria, Base Sequence, Cas9, Point mutation, RNA, pathogens, Cell Biology, molecular detection, 030104 developmental biology, Molecular Diagnostic Techniques, chemistry, Mutation, Viruses, Streptococcus pyogenes, CRISPR/Cas systems, Molecular Medicine, CRISPR-Cas Systems, DNA

Abstract

The Streptococcus pyogenes CRISPR/Cas system has found widespread applications as a gene‐editing and regulatory tool for the simultaneous delivery of the Cas9 protein and guide RNAs into the cell, thus making the recognition of specific DNA sequences possible. The recent study that shows that Cas9 can also bind to and cleave RNA in an RNA‐programmable manner is suggestive of potential utility of this system as a universal nucleic‐acid recognition tool. To increase the signal intensity of the CRISPR/Cas system, a signal amplification technique has to be exploited appropriately; this requirement is also a challenge for the detection of DNA or RNA. Furthermore, the CRISPR/Cas system may be used to detect point mutations or single‐nucleotide variants because of the specificity of the recognition between the target sequence and the CRISPR/Cas system. These lines of evidence make this technique capable of detecting pathogens during infection via analysis of their DNA or RNA. Thus, here we summarize applications of the CRISPR/Cas system to the recognition and detection of DNA and RNA molecules as well as the signal amplification. We also describe its potential ability to detect mutations and single‐nucleotide variants. Finally, we sum up its applications to testing for pathogens and potential barriers for its implementation.

Published

2018

19. Clustered Regularly Interspaced Short Palindromic Repeat (CRISPR)/CRISPR-Associated Endonuclease Cas9–Mediated Homology-Independent Integration for Generating Quality Control Materials for Clinical Molecular Genetic Testing

Author

Jiehong Xie, Yanxi Han, Jinming Li, Rongxue Peng, Guigao Lin, and Kuo Zhang

Subjects

Quality Control, 0301 basic medicine, medicine.medical_specialty, Computational biology, Biology, Pathology and Forensic Medicine, 03 medical and health sciences, chemistry.chemical_compound, symbols.namesake, 0302 clinical medicine, Plasmid, Genome editing, CRISPR-Associated Protein 9, Molecular genetics, medicine, Humans, CRISPR, Gene Knock-In Techniques, Genetic Testing, Gene Editing, Sanger sequencing, Base Sequence, Genome, Human, Cas9, Reproducibility of Results, Non-homologous end joining, HEK293 Cells, 030104 developmental biology, chemistry, 030220 oncology & carcinogenesis, Mutation, symbols, Molecular Medicine, CRISPR-Cas Systems, DNA

Abstract

Genome-edited human cell lines are important resources for producing quality control materials for clinical molecular genetic testing. Generating cell lines with defined mutations through homology-directed repair-based methods are inefficient and can lead to unwanted insertions and deletions in the target loci. Nonhomologous end joining in the clustered regularly interspaced short palindromic repeat (CRISPR)/CRISPR-associated endonuclease Cas9 (Cas9) system was harnessed to generate genome-engineered cell lines harboring target mutations. Donor plasmids containing target sites for the single guide RNA (sgRNA) and homologous DNA fragments harboring important cancer gene mutations were cotransfected with the Cas9/sgRNA vector into wild-type human cells. The introduced mutations were validated in-house and in 44 laboratories using various techniques, including next-generation sequencing. Exogenous sequences containing the target mutations were efficiently integrated into the ALK receptor tyrosine kinase (ALK) locus in HEK293T and A549 cells. Successful introduction of artificial mutations was confirmed via both Sanger sequencing and the amplification refractory mutation system. Results of external pilot testing revealed that the DNA samples derived from genome-edited cell lines were widely applicable across multiple platforms and laboratories. This study demonstrates that CRISPR/Cas9-induced nonhomologous end joining is a valuable and novel method for generating artificial mutants for use in quality control applications in clinical molecular genetics.

Published

2018

20. CRISPR/Cas9 Technology–Based Xenograft Tumors as Candidate Reference Materials for Multiple EML4-ALK Rearrangements Testing

Author

Ziyang Li, Rui Zhang, Kuo Zhang, Jiawei Zhang, Xin Yang, Guigao Lin, Jinming Li, and Rongxue Peng

Subjects

0301 basic medicine, Oncogene Proteins, Fusion, Computational biology, In situ hybridization, Biology, Real-Time Polymerase Chain Reaction, Polymorphism, Single Nucleotide, Sensitivity and Specificity, Cell Line, Pathology and Forensic Medicine, Mice, 03 medical and health sciences, 0302 clinical medicine, hemic and lymphatic diseases, medicine, Animals, Humans, CRISPR, Anaplastic lymphoma kinase, Genetic Testing, In Situ Hybridization, Fluorescence, Gene Editing, Gene Rearrangement, medicine.diagnostic_test, Cas9, High-Throughput Nucleotide Sequencing, Reproducibility of Results, Assay sensitivity, Gene rearrangement, Immunohistochemistry, Molecular biology, Disease Models, Animal, 030104 developmental biology, 030220 oncology & carcinogenesis, Gene Targeting, Heterografts, Molecular Medicine, CRISPR-Cas Systems, Fluorescence in situ hybridization

Abstract

The echinoderm microtubule-associated protein-like 4 and anaplastic lymphoma kinase (ALK) receptor tyrosine kinase (EML4-ALK) rearrangement is an important biomarker that plays a pivotal role in therapeutic decision making for non-small-cell lung cancer (NSCLC) patients. Ensuring accuracy and reproducibility of EML4-ALK testing by fluorescence in situ hybridization, immunohistochemistry, RT-PCR, and next-generation sequencing requires reliable reference materials for monitoring assay sensitivity and specificity. Herein, we developed novel reference materials for various kinds of EML4-ALK testing. CRISPR/Cas9 was used to edit various NSCLC cell lines containing EML4-ALK rearrangement variants 1, 2, and 3a/b. After s.c. inoculation, the formalin-fixed, paraffin-embedded (FFPE) samples from xenografts were prepared and tested for suitability as candidate reference materials by fluorescence in situ hybridization, immunohistochemistry, RT-PCR, and next-generation sequencing. Sample validation and commutability assessments showed that all types of FFPE samples derived from xenograft tumors have typical histological structures, and EML4-ALK testing results were similar to the clinical ALK-positive NSCLC specimens. Among the four methods for EML4-ALK detection, the validation test showed 100% concordance. Furthermore, these novel FFPE reference materials showed good stability and homogeneity. Without limitations on variant types and production, our novel FFPE samples based on CRISPR/Cas9 editing and xenografts are suitable as candidate reference materials for the validation, verification, internal quality control, and proficiency testing of EML4-ALK detection.

Published

2017

21. Technical Validation of a Next-Generation Sequencing Assay for Detecting Clinically Relevant Levels of Breast Cancer–Related Single-Nucleotide Variants and Copy Number Variants Using Simulated Cell-Free DNA

Author

Jiehong Xie, Zhao Meiru, Tian Lu, Kuo Zhang, Jiansheng Ding, Xin Yi, Ziyang Li, Lang Yi, Xin Yang, Guigao Lin, Ling Yang, Dongdong Li, Yuxing Chu, Lucheng Zhang, Dan Li, Yu Fu, Qisheng Wu, Rui Zhang, Rongxue Peng, Jinming Li, Liu Tao, and Yanxi Han

Subjects

0301 basic medicine, DNA Copy Number Variations, Mutant allele, Breast Neoplasms, Biology, Polymorphism, Single Nucleotide, Sensitivity and Specificity, DNA sequencing, Pathology and Forensic Medicine, 03 medical and health sciences, Breast cancer, medicine, Humans, Digital polymerase chain reaction, Copy-number variation, Gene, Genetics, High-Throughput Nucleotide Sequencing, Reproducibility of Results, medicine.disease, Plasma.cfDNA, 030104 developmental biology, Cell-free fetal DNA, Molecular Medicine, Female, Cell-Free Nucleic Acids

Abstract

Next-generation sequencing (NGS) is commonly used in a clinical setting for diagnostic and prognostic testing of genetic mutations to select optimal targeted therapies. Herein, we describe the development of a custom NGS assay for detecting single-nucleotide variants (SNVs) and copy number variations (CNVs) in a panel of 51 genes related to breast cancer. We designed and implemented a validation strategy in accordance with principles and guidelines developed by the Next-Generation Sequencing: Standardization of Clinical Testing work group using artificial, cell-free DNA (cfDNA) with mutant fragments prepared in a simple, rapid, and cost-effective manner. For SNV detection, our test had 96.30% sensitivity at mutant allele frequency ≥0.5% with high specificity (99.9997%) and accuracy (99.9996%). For CNV detection, the approach had 95.83% sensitivity for copy numbers at 1.25× (25.6% extra copies) with high specificity (99.77%) and accuracy (99.76%). In addition, our NGS-based assay demonstrated high intrarun and interrun reproducibility, high consistency compared to digital PCR, and a low cross-contamination rate. An overall assessment using cfDNA and plasma cfDNA samples demonstrated our custom NGS assay yields a reliable and robust detection sensitivity with a mutant allele frequency as low as 0.5% for SNVs and copy number of 1.25× for CNVs.

Published

2017

22. RCasFISH: CRISPR/dCas9-Mediated in Situ Imaging of mRNA Transcripts in Fixed Cells and Tissues

Author

Kun Chen, Jinming Li, Rongxue Peng, Meng Wang, Qisheng Wu, and Rui Zhang

Subjects

Tissue Fixation, In situ hybridization, 010402 general chemistry, Real-Time Polymerase Chain Reaction, 01 natural sciences, Analytical Chemistry, Gene expression, medicine, Tumor Cells, Cultured, CRISPR, Humans, RNA, Messenger, Gene, In Situ Hybridization, Fluorescence, Messenger RNA, Microscopy, Confocal, medicine.diagnostic_test, Chemistry, Lasers, 010401 analytical chemistry, RNA, 0104 chemical sciences, Cell biology, Real-time polymerase chain reaction, CRISPR-Cas Systems, Fluorescence in situ hybridization

Abstract

Effective characterization and imaging of endogenous RNA transcripts have important value in the diagnosis, treatment, and prognosis of diseases. Traditional qRT-PCR as a liquid-based RNA detection method might lead to false-negative results due to the admixture of too many nontarget cells. Also, many in situ RNA imaging methods were hindered by long turnaround time and insufficient signals. Here, we describe and evaluate a CRISPR/dCas9-MS2-based RNA fluorescence in situ hybridization assay (RCasFISH) for in situ amplified imaging and quantification of RNA transcripts in fixed cells as well as formalin-fixed, paraffin-embedded (FFPE) tissue sections at a single-molecular level in individual cells. Compared to single molecular FISH (smFISH), RCasFISH yields brighter dot signals and a better signal-to-noise ratio (SNR) with lower costs and less than 1.5 h of hybridization. In addition, by using human epidermal growth factor receptor 2 (HER2) as a model, we quantified individual HER2 mRNA molecules in clinical breast cancer FFPE tissue sections and demonstrated its potential to resolve FISH-equivocal cases. Therefore, RCasFISH may provide a new approach for gene expression studies in basic research and hold the potential for molecular diagnostic applications.

Published

2019

23. Standardization of BCR-ABL1 quantification on the international scale in China using locally developed secondary reference panels

Author

Rui Zhang, Rongxue Peng, Qisheng Wu, Lihua Bao, Jiawei Zhang, Jinming Li, and Yu Fu

Subjects

0301 basic medicine, Quality Control, Cancer Research, China, Standardization, Computer science, International scale, Fusion Proteins, bcr-abl, World health, 03 medical and health sciences, Bcr abl1, 0302 clinical medicine, hemic and lymphatic diseases, External quality assessment, Genetics, Secondary reference, Humans, Molecular Biology, Reference standards, Gene Expression Regulation, Leukemic, Reverse Transcriptase Polymerase Chain Reaction, Cell Biology, Hematology, Reference Standards, Manufacturing engineering, 030104 developmental biology, Multicenter study, 030220 oncology & carcinogenesis

Abstract

For patients with chronic myeloid leukemia, reverse transcription quantitative polymerase chain reaction is widely used in laboratories to quantify BCR-ABL1 fusion gene transcripts for disease management. Many efforts have been made to standardize the BCR-ABL1 testing assay, including the primary and secondary reference reagents, but the secondary standards have not been developed and used in the standardization program in China. With the use of armored RNA technology, armored RNA of BCR-ABL1 and control genes was manufactured to prepare the secondary reference material anchored to the World Health Organization primary reference calibrators for standardization of BCR-ABL1 testing assays. The secondary reference was sent to 30 laboratories in China for validation. Data from an external quality assessment after the standardization process were collected and analyzed as well. The assigned %BCR-ABL1/ABL1IS values of the four levels of the secondary material panels were 0.0118, 0.1345, 1.3808, and 19.4266, respectively. In validation trials, 70.0% (21/30) of laboratories obtained valid conversion factors for the BCR-ABL1 assay. All valid conversion factors from 11 international scale laboratories were equivalent to their respective previous values. External quality assessment data indicated that the accuracy and precision between laboratories were improved. Moreover, the quantity of the panels is abundant to be used as quality control samples for monitoring the shift of data. In this study, we established a secondary genetic reference panel for BCR-ABL1 quantification. This study will play a role in facilitating the worldwide dissemination of the international scale, especially in promoting the standardization of molecular monitoring in China.

Published

2019

24. Continual Improvement of the Reliability of EML4-ALK Rearrangement Detection in Non-Small-Cell Lung Cancer: A Long-Term Comparison of ALK Detection in China

Author

Rongxue, Peng, Rui, Zhang, Jiawei, Zhang, Ping, Tan, Yanxi, Han, Kuo, Zhang, Guigao, Lin, Jiehong, Xie, and Jinming, Li

Subjects

Gene Rearrangement, China, Laboratory Proficiency Testing, Lung Neoplasms, Oncogene Proteins, Fusion, Reverse Transcriptase Polymerase Chain Reaction, Mice, Nude, Reproducibility of Results, Quality Improvement, Xenograft Model Antitumor Assays, Tumor Burden, Mice, HEK293 Cells, Carcinoma, Non-Small-Cell Lung, Cell Line, Tumor, Animals, Humans, Anaplastic Lymphoma Kinase, Female, CRISPR-Cas Systems, Precision Medicine, In Situ Hybridization, Fluorescence

Abstract

The results of EML4-ALK testing are critical to manage ALK tyrosine kinase receptor inhibitor treatment. Thus, the accurate detection of ALK rearrangement is increasingly becoming a matter of serious concern. To address this issue, a long-term EML4-ALK proficiency testing (PT) scheme was launched in China in 2015, serving as an educational tool for assessing and improving the testing quality of EML4-ALK fusion detection. Responses across 20 different PT samples interrogating three different variants and wild-type samples were collected between 2015 and 2019. Performance was analyzed by evaluating the detection methods, kits, and pre-analytic practices used to further display the landscape of changing conditions of the reliability of EML4-ALK testing. During the 5 years, 3224 results reported from 988 laboratories were evaluated, with an overall error rate of 5.36%. Along with an increasing number of participating laboratories, the error rate within each of the different methods showed a significantly downward trend over the years. No obvious differences in the error rates were found regarding the testing methods or kit manufacturers. Moreover, the individual performance of the laboratories improved when they participated in more PT scheme rounds. The data demonstrated that the performance of individual Chinese laboratories for EML4-ALK testing continuously improved over time by participating PT schemes, regardless of their method. However, care must be taken in standardized operations and validations.

Published

2019

25. External Quality Assurance of Current Technology for the Testing of Cancer-Associated Circulating Free DNA Variants

Author

Jinming Li, Nalishia Pillay, Tony Badrick, Kwang Hong Tay, Martin Horan, Rui Zhang, Sze Yee Chai, Li Zhou, and Rongxue Peng

Subjects

0301 basic medicine, Oncology, Cancer Research, medicine.medical_specialty, Genotype, Quality Assurance, Health Care, Pilot Projects, Polymerase Chain Reaction, Pathology and Forensic Medicine, Circulating Tumor DNA, 03 medical and health sciences, 0302 clinical medicine, Internal medicine, Medicine, Humans, Digital polymerase chain reaction, Liquid biopsy, Genotyping, Allele frequency, business.industry, Liquid Biopsy, Cancer, High-Throughput Nucleotide Sequencing, General Medicine, Sequence Analysis, DNA, medicine.disease, 030104 developmental biology, Circulating free DNA, 030220 oncology & carcinogenesis, Multiple comparisons problem, business, Quality assurance

Abstract

Liquid biopsy testing is rapidly emerging as a diagnostic means of identifying circulating free DNA (cfDNA) disease-associated variants. However, the reporting of cfDNA variants remains inconsistent due in part to the application of multiple testing pipelines which raise uncertainty about current cfDNA detection efficiency. External quality assurance (EQA) programs are required to monitor, evaluate and help improve laboratory performance for cfDNA variant detection and in clinical interpretation. This study therefore evaluated the performance of diagnostic laboratories currently performing cfDNA testing in China, Australia and New Zealand. A total of 89 laboratories participated in this EQA program. Reference testing material comprised of cfDNA manufactured to contain six different genotypes in four different genes (EGFR, KRAS, BRAF, NRAS). The predicted genotypic variant allelic frequencies ranged between 0.5% - 2.5%. Proficiency testing used a z-score on the laboratory consensus allelic frequency data to compare laboratory performance for the detection of the different genotypes. Allelic frequency genotyping data were received from 88 of the 89 laboratories. Next generation sequencing and digital PCR testing platforms were primarily used by participants in this pilot EQA. The average consensus data for each cfDNA genotype identified allelic frequencies ranging between 0.39% - 4.4%. Z-score proficiency testing found that >92% of clinical laboratories were concordant for detecting the cfDNA variants. The data from this pilot study suggest that current cfDNA testing platforms can detect cfDNA allelic frequency variants from 0.39% and above with high levels of confidence. In addition, these data highlight the importance of laboratories enrolling on EQA programs so that proficiency in cfDNA diagnostic testing can be determined and potential sources of error identified and addressed.

Published

2019

26. Clinician-friendly reports of molecular measurable residual disease monitoring in acute promyelocytic leukemia

Author

Yu Fu, Qisheng Wu, Jiawei Zhang, Rui Zhang, Rongxue Peng, Kun Chen, and Jinming Li

Subjects

Acute promyelocytic leukemia, medicine.medical_specialty, Neoplasm, Residual, Real-Time Polymerase Chain Reaction, 03 medical and health sciences, 0302 clinical medicine, Leukemia, Promyelocytic, Acute, hemic and lymphatic diseases, medicine, Electronic Health Records, Humans, Medical physics, Clinical significance, Monitoring, Physiologic, business.industry, Hematology, General Medicine, Disease monitoring, Tissue sampling, medicine.disease, body regions, Clinical Practice, 030220 oncology & carcinogenesis, Clinical case, business, 030215 immunology

Abstract

Molecular measurable residual disease (MRD) monitoring based on real-time quantitative reverse transcription PCR (RT-qPCR) plays an important role in acute promyelocytic leukemia (APL) management, but the performance status of clinical reports is unknown. This study focuses on the specific elements in molecular MRD monitoring report and their impact on clinical decision-making. The participating laboratories were asked to submit real and formal clinical reports for mock samples panel with APL clinical case. The MRD-specific elements were analyzed and summarized. The significance of longitudinal MRD monitoring curve and the missing MRD-specific elements for clinical decision-making were assessed. MRD-specific elements were significantly missing in clinical reports. The element “testing results” existed great inconsistencies in the written form of testing items and data. The longitudinal MRD monitoring curve of false-negative or false-positive MRD result was obviously different from all-correct. It not only identified MRD time point of tissue sampling relative to treatment and ensured the reliability of the negative MRD results, but also gave MRD diagnosis, clinical interpretation, and further recommendation. Clinician-friendly reports with MRD-specific elements can better serve clinical practice. The correctly intuitive results and clinically important MRD-specific elements can provide a good description of the reliability and clinical significance of MRD results.

Published

2018

27. Potential pitfalls of CRISPR/Cas9-mediated genome editing

Author

Guigao Lin, Jinming Li, and Rongxue Peng

Subjects

0301 basic medicine, Genetic enhancement, Biology, Biochemistry, 03 medical and health sciences, Synthetic biology, Genome editing, Humans, CRISPR, Guide RNA, Molecular Biology, Genetics, Binding Sites, Models, Genetic, Genome, Human, Cas9, Reproducibility of Results, Gene targeting, Genetic Therapy, Cell Biology, 030104 developmental biology, Gene Targeting, Human genome, CRISPR-Cas Systems, Genetic Engineering, RNA, Guide, Kinetoplastida

Abstract

Recently, a novel technique named the clustered regularly interspaced short palindromic repeat (CRISPR)/CRISPR-associated protein (Cas)9 system has been rapidly developed. This genome editing tool has improved our ability tremendously with respect to exploring the pathogenesis of diseases and correcting disease mutations, as well as phenotypes. With a short guide RNA, Cas9 can be precisely directed to target sites, and functions as an endonuclease to efficiently produce breaks in DNA double strands. Over the past 30 years, CRISPR has evolved from the 'curious sequences of unknown biological function' into a promising genome editing tool. As a result of the incessant development in the CRISPR/Cas9 system, Cas9 co-expressed with custom guide RNAs has been successfully used in a variety of cells and organisms. This genome editing technology can also be applied to synthetic biology, functional genomic screening, transcriptional modulation and gene therapy. However, although CRISPR/Cas9 has a broad range of action in science, there are several aspects that affect its efficiency and specificity, including Cas9 activity, target site selection and short guide RNA design, delivery methods, off-target effects and the incidence of homology-directed repair. In the present review, we highlight the factors that affect the utilization of CRISPR/Cas9, as well as possible strategies for handling any problems. Addressing these issues will allow us to take better advantage of this technique. In addition, we also review the history and rapid development of the CRISPR/Cas system from the time of its initial discovery in 2012.

Published

2015

28. The miR-21 potential of serving as a biomarker for liver diseases in clinical practice.

Author

Jiawei Zhang, Dandan Li, Rui Zhang, Peng Gao, Rongxue Peng, and Jinming Li

Subjects

BIOMARKERS, LIVER diseases, PROGNOSIS, CIRRHOSIS of the liver, MICRORNA, TUMOR markers, GENE regulatory networks

Abstract

The role of miR-21 in the pathogenesis of various liver diseases, together with the possibility of detecting microRNA in the circulation, makes miR-21 a potential biomarker for noninvasive detection. In this review, we summarize the potential utility of extracellular miR-21 in the clinical management of hepatic disease patients and compared it with the current clinical practice. MiR-21 shows screening and prognostic value for liver cancer. In liver cirrhosis, miR-21 may serve as a biomarker for the differentiating diagnosis and prognosis. MiR-21 is also a potential biomarker for the severity of hepatitis. We elucidate the disease condition under which miR-21 testing can reach the expected performance. Though miR-21 is a key regulator of liver diseases, microRNAs coordinate with each other in the complex regulatory network. As a result, the performance of miR-21 is better when combined with other microRNAs or classical biomarkers under certain clinical circumstances. [ABSTRACT FROM AUTHOR]

Published

2020

29. Correction: External Quality Assessment of Molecular Detection of Ebola Virus in China

Author

Lei Zhang, Kuo Zhang, Rui Zhang, Guojing Wang, Yu Sun, Le Chang, Rongxue Peng, Tingting Jia, Mingju Hao, Dong Zhang, Jinming Li, and Guigao Lin

Subjects

China, Multidisciplinary, Ebola virus, Quality Assurance, Health Care, business.industry, lcsh:R, Library science, lcsh:Medicine, Correction, medicine.disease_cause, Ebolavirus, Virology, External quality assessment, Medicine, Humans, lcsh:Q, business, lcsh:Science, DNA Probes, Laboratories, DNA Primers

Abstract

In 2014, Ebola hemorrhagic fever broke out in West Africa. As contact between China and West Africa is frequent, the possibility that Ebola virus would enter China was high. Thus, an external assessment of the quality of Ebola virus detection was organized by the National Center for Clinical Laboratories in China. Virus-like particles encapsulating known sequences of epidemic strains of Ebola virus from 2014 were prepared as positive quality controls. The sample panel, which was composed of seven positive and three negative samples, was dispatched to 19 laboratories participating in this assessment of Ebola virus detection. Accurate detection was reported at 14 of the 19 participating laboratories, with a sensitivity of 91.43% and a specificity of 100%. Four participants (21.05%) reported false-negative results and were classified as "acceptable." One participant (5.26%) did not detect any positive samples and was thus classified as "improvable." Based on the results returned, the ability to detect weakly positive Ebola specimens should be improved. Furthermore, commercial assays and the standard primers offered by the Chinese Centers for Disease Control and Prevention were found to be most accurate and dependable for Ebola detection. A two-target detection approach is recommended for Ebola screening; this approach could reduce the probability of false-negative results. Additionally, standardization of operations and punctual adjustment of instruments are necessary for the control and prevention of Ebola virus.

Published

2016

30. Reliability Assurance of Detection of EML4-ALK Rearrangement in Non-Small Cell Lung Cancer: The Results of Proficiency Testing in China

Author

Jiansheng Ding, Yulong Li, Jinming Li, Kuo Zhang, Rongxue Peng, Han Yanxi, Guigao Lin, Rui Zhang, and Guojing Wang

Subjects

0301 basic medicine, Pulmonary and Respiratory Medicine, Oncology, medicine.medical_specialty, China, Laboratory Proficiency Testing, Lung Neoplasms, Oncogene Proteins, Fusion, Mice, Nude, Bioinformatics, law.invention, 03 medical and health sciences, Mice, 0302 clinical medicine, law, Internal medicine, Carcinoma, Non-Small-Cell Lung, Proficiency testing, medicine, Tumor Cells, Cultured, Animals, Humans, ALK Rearrangement, Lung cancer, Genotyping, Polymerase chain reaction, In Situ Hybridization, Fluorescence, Gene Rearrangement, medicine.diagnostic_test, business.industry, Reverse Transcriptase Polymerase Chain Reaction, Reproducibility of Results, medicine.disease, Immunohistochemistry, Xenograft Model Antitumor Assays, Reverse transcriptase, 030104 developmental biology, 030220 oncology & carcinogenesis, Biological Assay, Female, Non small cell, business, Fluorescence in situ hybridization

Abstract

Introduction Currently, several approaches are being used to detect echinoderm microtubule associated protein like 4 gene ( EML4 )–anaplastic lymphoma receptor tyrosine kinase gene ( ALK ) rearrangement, but the performance of laboratories in China is unknown. To evaluate the proficiency of different laboratories in detecting EML4-ALK rearrangement, we organized a proficiency test (PT). Methods We prepared formalin-fixed, paraffin-embedded samples derived from the xenograft tumor tissue of three non–small cell lung cancer cell lines with different EML4-ALK rearrangements and used PTs to evaluate the detection performance of laboratories in China. Results We received results from 94 laboratories that used different methods. Of the participants, 75.53% correctly identified all samples in the PT panel. Among the errors made by participants, false-negative errors were likely to occur. According to the methodology applied, 82.86%, 76.67%, 77.78%, and 66.67% of laboratories using reverse transcriptase polymerase chain reaction, fluorescence in situ hybridization, next-generation sequencing, and immunohistochemical analysis, respectively, could analyze all the samples correctly. Moreover, we have found that the laboratories' genotyping capacity is high, especially for variant 3. Conclusion Our PT survey revealed that the performance and methodological problems of laboratories must be addressed to further increase the reproducibility and accuracy of detection of EML4 - ALK rearrangement to ensure reliable results for selection of appropriate patients.

Published

2016

31. A novel cell line generated using the CRISPR/Cas9 technology as universal quality control material for KRAS G12V mutation testing

Author

Jiehong Xie, Yu Fu, Yanxi Han, Rongxue Peng, Peng Gao, Qisheng Wu, Shiyu Jia, Jinming Li, Rui Zhang, Guigao Lin, Kuo Zhang, and Jiansheng Ding

Subjects

0301 basic medicine, Microbiology (medical), DNA Mutational Analysis, Clinical Biochemistry, Glycine, Computational biology, Gene mutation, Biology, Transfection, medicine.disease_cause, Cell Line, Proto-Oncogene Proteins p21(ras), 03 medical and health sciences, symbols.namesake, 0302 clinical medicine, medicine, Humans, Immunology and Allergy, CRISPR, Digital polymerase chain reaction, Research Articles, Sanger sequencing, Cas9, Biochemistry (medical), Public Health, Environmental and Occupational Health, Valine, Hematology, Medical Laboratory Technology, HEK293 Cells, 030104 developmental biology, 030220 oncology & carcinogenesis, Mutation, Mutation (genetic algorithm), symbols, Mutation testing, KRAS, CRISPR-Cas Systems

Abstract

Background KRAS mutations are the key indicator for EGFR monoclonal antibody-targeted therapy and acquired drug resistance, and their accurate detection is critical to the clinical decision-making of colorectal cancer. However, no proper quality control material is available for the current detection methods, particularly next-generation sequencing (NGS). The ideal quality control material for NGS needs to provide both the tumor mutation gene and the matched background genomic DNA, which is uncataloged in public databases, to accurately distinguish germline polymorphisms and somatic mutations. Methods We developed a novel KRAS G12V mutant cell line using the clustered regularly interspaced short palindromic repeat (CRISPR)/CRISPR-associated protein 9 (Cas9) technique to make up for the deficiencies in existing quality control material and further validated the feasibility of the cell line as quality control material by amplification refractory mutation system (ARMS), Sanger sequencing, digital PCR (dPCR), and NGS. Results We verified that the edited cell line specifically had the G12V mutation, and the validation results presented a high consistency among the four methods of detection. The three cell lines screened contained the G12V mutation and the mutation allele fractions of G12V-1, G12V-2, and G12V-3 were 52.01%, 82.06%, and 17.29%, respectively. Conclusion The novel KRAS G12V cell line generated using the CRISPR/Cas9 gene editing system is suitable as a quality control material for all current detection methods and provides a new direction in the development of quality control material.

Published

2018

32. Synthetic Circulating Cell-free DNA as Quality Control Materials for Somatic Mutation Detection in Liquid Biopsy for Cancer.

Author

Rui Zhang, Rongxue Peng, Ziyang Li, Peng Gao, Shiyu Jia, Xin Yang, Jiansheng Ding, Yanxi Han, Jiehong Xie, and Jinming Li

Published

2017

33. External Quality Assessment of Molecular Detection of Ebola Virus in China

Author

Guojing Wang, Yu Sun, Dong Zhang, Jinming Li, Lei Zhang, Rui Zhang, Guigao Lin, Le Chang, Rongxue Peng, Kuo Zhang, Tingting Jia, and Mingju Hao

Subjects

Ebolavirus, Weakly positive, Multidisciplinary, Ebola virus, business.industry, viruses, lcsh:R, virus diseases, lcsh:Medicine, medicine.disease_cause, Virology, Disease control, West africa, Ebola Hemorrhagic Fever, External quality assessment, medicine, lcsh:Q, business, lcsh:Science, Research Article

Abstract

In 2014, Ebola hemorrhagic fever broke out in West Africa. As contact between China and West Africa is frequent, the possibility that Ebola virus would enter China was high. Thus, an external assessment of the quality of Ebola virus detection was organized by the National Center for Clinical Laboratories in China. Virus-like particles encapsulating known sequences of epidemic strains of Ebola virus from 2014 were prepared as positive quality controls. The sample panel, which was composed of seven positive and three negative samples, was dispatched to 19 laboratories participating in this assessment of Ebola virus detection. Accurate detection was reported at 14 of the 19 participating laboratories, with a sensitivity of 91.43% and a specificity of 100%. Four participants (21.05%) reported false-negative results and were classified as “acceptable.” One participant (5.26%) did not detect any positive samples and was thus classified as “improvable.” Based on the results returned, the ability to detect weakly positive Ebola specimens should be improved. Furthermore, commercial assays and the standard primers offered by the Chinese Centers for Disease Control and Prevention were found to be most accurate and dependable for Ebola detection. A two-target detection approach is recommended for Ebola screening; this approach could reduce the probability of false-negative results. Additionally, standardization of operations and punctual adjustment of instruments are necessary for the control and prevention of Ebola virus.