Your search keyword '"Immunoglobulin heavy chain"' showing total 4,433 results

1. Comparative analysis of a novel next-generation sequencing-based IGH clonality assay for measurable residual disease detection in pediatric B-cell acute lymphoblastic leukemia patients.

Author

Park, Min-Seung, Ju, Hee Young, Lee, Ji Won, Yoo, Keon Hee, Kim, Hee-Jin, Cho, Duck, and Kim, Hyun-Young

Abstract

AbstractMeasurable residual disease (MRD) is critical in guiding therapeutic strategies for B-cell acute lymphoblastic leukemia (B-ALL). This study evaluated the performance of a novel next-generation sequencing-based Celemics IGH assay (CM-IGH; Celemics, Seoul, Korea) compared with the LymphoTrack® IGH FR1 assay (LT-IGH; Invivoscribe Technologies, USA) and multiparameter flow cytometry (MFC). A total of 31 diagnostic and 60 follow-up bone marrow aspirate samples, all from the same 31 pediatric patients with B-ALL, were analyzed using the CM-IGH and LT-IGH assays on the MiSeq platform, as well as MFC according to EuroFlow guidelines. Initial IGH clonality was detected in 83.9% of CM-IGH samples and 90.3% of LT-IGH samples (p = 0.060). MRD positivity rates in follow-up samples were 74.5% for CM-IGH, 61.1% for LT-IGH, and 56.7% for MFC. CM-IGH showed concordance rates of 78.3% with LT-IGH and 68.1% with MFC, while LT-IGH demonstrated an 81.5% concordance rate with MFC. The correlation coefficients (r) of MRD levels were 0.831 between CM-IGH and LT-IGH, 0.702 between CM-IGH and MFC, and 0.776 between LT-IGH and MFC. The CM-IGH assay demonstrates substantial concordance with LT-IGH and MFC in detecting MRD in pediatric patients with B-ALL, highlighting the complementary value of IGH clonality assays and MFC. [ABSTRACT FROM AUTHOR]

Published

2025

2. Interpretable deep learning reveals the role of an E-box motif in suppressing somatic hypermutation of AGCT motifs within human immunoglobulin variable regions.

Author

Tambe, Abhik, MacCarthy, Thomas, and Pavri, Rushad

Subjects

DEEP learning, IMMUNOGLOBULIN class switching, HUMORAL immunity, MACHINE learning, B cells, IMMUNOGLOBULIN heavy chains, NUCLEOTIDE sequence

Abstract

Introduction: Somatic hypermutation (SHM) of immunoglobulin variable (V) regions by activation induced deaminase (AID) is essential for robust, longterm humoral immunity against pathogen and vaccine antigens. AID mutates cytosines preferentially within WRCH motifs (where W=A or T, R=A or G and H=A, C or T). However, it has been consistently observed that the mutability of WRCH motifs varies substantially, with large variations in mutation frequency even between multiple occurrences of the same motif within a single V region. This has led to the notion that the immediate sequence context of WRCH motifs contributes to mutability. Recent studies have highlighted the potential role of local DNA sequence features in promoting mutagenesis of AGCT, a commonly mutated WRCH motif. Intriguingly, AGCT motifs closer to 5' ends of V regions, within the framework 1 (FW1) sub-region1, mutate less frequently, suggesting an SHM-suppressing sequence context. Methods: Here, we systematically examined the basis of AGCT positional biases in human SHM datasets with DeepSHM, a machine-learning model designed to predict SHM patterns. This was combined with integrated gradients, an interpretability method, to interrogate the basis of DeepSHM predictions. Results: DeepSHM predicted the observed positional differences in mutation frequencies at AGCT motifs with high accuracy. For the conserved, lowly mutating AGCT motifs in FW1, integrated gradients predicted a large negative contribution of 5'C and 3'G flanking residues, suggesting that a CAGCTG context in this location was suppressive for SHM. CAGCTG is the recognition motif for Ebox transcription factors, including E2A, which has been implicated in SHM. Indeed, we found a strong, inverse relationship between E-box motif fidelity and mutation frequency. Moreover, E2A was found to associate with the V region locale in two human B cell lines. Finally, analysis of human SHM datasets revealed that naturally occurring mutations in the 3'G flanking residues, which effectively ablate the E-box motif, were associated with a significantly increased rate of AGCT mutation. Discussion: Our results suggest an antagonistic relationship between mutation frequency and the binding of E-box factors like E2A at specific AGCT motif contexts and, therefore, highlight a new, suppressive mechanism regulating local SHM patterns in human V regions. [ABSTRACT FROM AUTHOR]

Published

2024

3. The aryl hydrocarbon receptor differentially modulates the expression profile of antibody isotypes in a human B-cell line.

Author

Bhakta-Yadav, Mili S, Burra, Kaulini, Alhamdan, Nasser, Allex-Buckner, Clayton P, and Sulentic, Courtney E W

Subjects

*ARYL hydrocarbon receptors, *B cells, *GENE expression, *IMMUNOGLOBULIN heavy chains, *IMMUNOGLOBULIN class switching, *ANTIBODY formation

Abstract

2,3,7,8‐Tetrachlorodibenzo‐p‐dioxin (TCDD) is a persistent environmental contaminant and high affinity ligand for the aryl hydrocarbon receptor (AhR). In animal models, AhR activation by TCDD generally inhibits antibody secretion. However, it is less clear if this translates to human antibody production. Using a human Burkitt lymphoma B-cell line (CL-01) that can be stimulated to secrete Ig and undergo class switch recombination to other Ig isotypes, the current study evaluated the effects of AhR activation or antagonism on the human Ig isotypic expression profile with CD40L+IL-4 stimulation. Our results suggest that AhR agonists (TCDD and indirubin) have little to no effect on IgM or IgA secretion, which were also not induced with stimulation. However, AhR activation significantly inhibited stimulation-induced IgG secretion, an effect reversed by the AhR antagonist CH223191. Evaluation of Ig heavy chain (IgH) constant region gene expression (ie Cμ, Cγ1-4, Cα1-2, and Cε that encode for IgM, IgG1-4, IgA1-2, and IgE, respectively) demonstrated differential effects. While Cμ and Cα2 transcripts were unaffected by stimulation or AhR agonists, AhR activation significantly inhibited stimulation-induced Cγ2-4 and Cε mRNA transcripts, which was reversed by AhR antagonism. Notably, AhR antagonism in the absence of exogenous AhR ligands significantly increased IgG and IgA secretion as well as the expression of Cγ2-4 and Cε. These results suggest that modulation of AhR activity differentially alters the IgH isotypic expression profile and antibody secretion that may be partly dependent on cellular stimulation. Since a variety of chemicals from anthropogenic, industrial, pharmaceutical, dietary, and bacterial sources bind the AhR, the ability of environmental exposures to alter AhR activity (i.e. activate or inhibit) may have a direct influence on immune function and antibody-relevant disease conditions. [ABSTRACT FROM AUTHOR]

Published

2024

4. Interpretable deep learning reveals the role of an E-box motif in suppressing somatic hypermutation of AGCT motifs within human immunoglobulin variable regions

Author

Abhik Tambe, Thomas MacCarthy, and Rushad Pavri

Subjects

somatic hypermutation (SHM), activation induced deaminase (AID), immunoglobulin heavy chain, deep learning, integrated gradients, E-box transcription factors, Immunologic diseases. Allergy, RC581-607

Abstract

IntroductionSomatic hypermutation (SHM) of immunoglobulin variable (V) regions by activation induced deaminase (AID) is essential for robust, long-term humoral immunity against pathogen and vaccine antigens. AID mutates cytosines preferentially within WRCH motifs (where W=A or T, R=A or G and H=A, C or T). However, it has been consistently observed that the mutability of WRCH motifs varies substantially, with large variations in mutation frequency even between multiple occurrences of the same motif within a single V region. This has led to the notion that the immediate sequence context of WRCH motifs contributes to mutability. Recent studies have highlighted the potential role of local DNA sequence features in promoting mutagenesis of AGCT, a commonly mutated WRCH motif. Intriguingly, AGCT motifs closer to 5’ ends of V regions, within the framework 1 (FW1) sub-region1, mutate less frequently, suggesting an SHM-suppressing sequence context.MethodsHere, we systematically examined the basis of AGCT positional biases in human SHM datasets with DeepSHM, a machine-learning model designed to predict SHM patterns. This was combined with integrated gradients, an interpretability method, to interrogate the basis of DeepSHM predictions.ResultsDeepSHM predicted the observed positional differences in mutation frequencies at AGCT motifs with high accuracy. For the conserved, lowly mutating AGCT motifs in FW1, integrated gradients predicted a large negative contribution of 5’C and 3’G flanking residues, suggesting that a CAGCTG context in this location was suppressive for SHM. CAGCTG is the recognition motif for E-box transcription factors, including E2A, which has been implicated in SHM. Indeed, we found a strong, inverse relationship between E-box motif fidelity and mutation frequency. Moreover, E2A was found to associate with the V region locale in two human B cell lines. Finally, analysis of human SHM datasets revealed that naturally occurring mutations in the 3’G flanking residues, which effectively ablate the E-box motif, were associated with a significantly increased rate of AGCT mutation.DiscussionOur results suggest an antagonistic relationship between mutation frequency and the binding of E-box factors like E2A at specific AGCT motif contexts and, therefore, highlight a new, suppressive mechanism regulating local SHM patterns in human V regions.

Published

2024

5. Pitfalls in diagnosing a case of extranodal NK/T‐cell lymphoma with CD20 aberrant expression and IGH gene rearrangement.

Author

Liu, Chenxi, Li, Fan, Mao, Chunyan, Dangzeng, Zhuoma, and Wang, Lin

Subjects

*GENE rearrangement, *T-cell receptor genes, *CD20 antigen, *IMMUNOGLOBULIN heavy chains, *GENE expression, *B cells

Abstract

Extranodal NK/T‐cell lymphoma (ENKTL) is a subtype of non‐Hodgkin lymphoma mainly derived from NK cells and, uncommonly, T‐cells. A diagnostic challenge is presented when an atypical phenotype and gene rearrangement are encountered. Herein, we report a case of ENKTL with CD20 expression and IGH gene rearrangement, which is extremely rare. A 57‐year‐old female patient was seen in 2021 due to a nodule on her left leg and simultaneously impaired eyesight for 6 months. Skin biopsy and immunohistochemistry were performed. The lymphoid cells were positive for CD3, CD56, granzyme B, and TIA‐1, partially positive for CD2, and mildly positive for CD20. In situ hybridization for Epstein–Barr virus was positive. Molecular studies revealed immunoglobulin heavy chain (IGH) gene rearrangement, while no T‐cell receptor gene rearrangement was detected. The positron emission tomography scan showed that the lymphoma affected bilateral adrenal glands, pelvic cavity, peritoneal cavity, small intestine, skin, and subcutis of the bilateral lower extremities of the patient. Her disease progressed despite eight cycles of chemotherapy and radiation therapy. The importance of this case lies in the atypical phenotype and IGH gene rearrangements, necessitating comprehensive interpretation of clinicopathological data. [ABSTRACT FROM AUTHOR]

Published

2023

6. The dynamic TRβ/IGH CDR3 repertoire features in patients with liver transplantation.

Author

Junning Zhang, Zhenyu Liu, Guangyu Wang, Xueli Yang, Weiguo Sui, Haonan Guo, and Xianliang Hou

Subjects

*LIVER transplantation, *T cell receptors, *IMMUNOGLOBULIN heavy chains, *AMINO acid sequence, *NUCLEOTIDE sequencing

Abstract

Objective: At present, little is known about the immune mechanism of liver transplantation caused by decompensated cirrhosis. Lymphocytes play an essential important role in the immune rejection of liver transplantation. In this study, we aimed to comprehensively analyze changes in complementary determinant 3 (CDR3) repertoire of T cell receptor β chain (TRβ) and immunoglobulin heavy chain (IGH) in liver transplantation patients and healthy controls (HC). Methods: High-throughput sequencing technology was used to study the characteristics of TRβ/IGH CDR3 repertoire, and identify the amino acid sequences of TRβ and IGH associated with liver transplantation patients and HC. Results: We found that some TRβ and IGH CDR3 repertoire characteristics differed between liver transplant patients and HC. The diversity of TRβ CDR3 increased in the liver transplantation group. First and seven days after live transplantation patients showed a lower degree of T cell clone amplification compared to the HC group. The CDR3 repertoire of the TRβ/IGH chain was certainly biased in the use of some V, D, and J gene segments, TRβ/IGH V-J combined frequency was also skewed and TRβ CDR3 clonotypes were shared at a higher degree in the liver transplantation patients. Importantly, one amino acid sequence in the decompensated cirrhosis group was significantly higher than that in the healthy group. It should be noted that the frequency of some CDR3 sequences is closely correlated with the different stages of liver transplantation, and these sequences may play a key role in liver transplantation. Conclusion: Based on the above results, we can better understand the dynamic changes of TCβ/IGH CDR3 repertoire in patients during liver transplantation. [ABSTRACT FROM AUTHOR]

Published

2023

7. Single-Step IGHV Next-Generation Sequencing Detects Clonality and Somatic Hypermutation in Lymphoid Malignancies: A Phase III Diagnostic Accuracy Study.

Author

Gazzola, Anna, Navari, Mohsen, Mannu, Claudia, Donelli, Riccardo, Etebari, Maryam, and Piccaluga, Pier Paolo

Subjects

*DIAGNOSIS of blood diseases, *LYMPHATIC disease diagnosis, *SEQUENCE analysis, *PREDICTIVE tests, *EVIDENCE-based medicine, *CAPILLARY electrophoresis, *GENES, *RESEARCH funding, *DESCRIPTIVE statistics, *SENSITIVITY & specificity (Statistics), *CYTOLOGY, *PHENOTYPES

Abstract

Simple Summary: Clonality testing and somatic hypermutation analysis performed on B-cell receptor encoding genes are the most widely used molecular assays for lymphoma diagnostics. Currently, PCR-based methods standardized by the BIOMED2 consortium are regarded as the gold standard. In the last few years, new approaches based on next-generation sequencing (NGS) have been proposed and validated in phase I–II studies. Here, we present the first phase III diagnostic accuracy study, evaluating an NGS-based protocol (LymphoTrack® IGH assay, and LymphoTrack® IGH somatic hypermutation assay) compared to the gold standard. We formally documented a high diagnostic accuracy providing a clinical validation of the assays. Background: Multiplex PCR based on consensus primers followed by capillary electrophoresis and Sanger sequencing are considered as the gold standard method for the evaluation of clonality and somatic hypermutation in lymphoid malignancies. As an alternative, the next-generation sequencing (NGS) of immune receptor genes has recently been proposed as a solution, due to being highly effective and sensitive. Here, we designed a phase III diagnostic accuracy study intended to compare the current gold standard methods versus the first commercially available NGS approaches for testing immunoglobulin heavy chain gene rearrangements. Methods: We assessed IGH rearrangements in 68 samples by means of both the NGS approach (LymphoTrack® IGH assay, and LymphoTrack® IGH somatic hypermutation assay, run on Illumina MiSeq) and capillary electrophoresis/Sanger sequencing to assess clonality and somatic hypermutations (SHM). Results: In comparison to the routine capillary-based analysis, the NGS clonality assay had an overall diagnostic accuracy of 96% (63/66 cases). Other studied criteria included sensitivity (95%), specificity (100%), positive predictive value (100%) and negative predictive value (75%). In discrepant cases, the NGS results were confirmed by a different set of primers that provided coverage of the IGH leader sequence. Furthermore, there was excellent agreement of the SHM determination with both the LymphoTrack® FR1 and leader assays when compared to the Sanger sequencing analysis (84%), with NGS able to assess the SHM rate even in cases where the conventional approach failed. Conclusion: Overall, conventional Sanger sequencing and next-generation-sequencing-based clonality and somatic hypermutation analyses gave comparable results. For future use in a routine diagnostic workflow, NGS-based approaches should be evaluated prospectively and an analysis of cost-effectiveness should be performed. [ABSTRACT FROM AUTHOR]

Published

2023

8. Minimal Residual Disease Detection Using Gene Scanning Analysis, Fluorescent Fragment Analysis, and Capillary Electrophoresis for IgH Rearrangement in Adult B-Lineage Acute Lymphoblastic Leukemia: A Cross-Sectional Study

Author

Sepideh Shahkarami, Samareh Younesian, Shahrbano Rostami, Farzad Kompani, Davood Bashash, Seyed Mousavi, and Seyed Ghaffari

Subjects

acute lymphoblastic leukemia, capillary gel electrophoresis, immunoglobulin heavy chain, genescanning, minimal residual disease, Medicine, Science

Abstract

Objective: Minimal residual disease (MRD) is considered the greatest prognostic factor in acute lymphoblastic leukemia(ALL). MRD is a valuable tool for anticipating impending relapse and treatment response assessment. The objective ofthe present study was to investigate whether the detection of IgH gene rearrangement using polymerase chain reaction(PCR)-based GeneScan analysis could be a complementary method to monitor MRD along with the quantitative realtimePCR (qPCR).Materials and Methods: In this cross-sectional study, we valued the MRD levels, based on the GeneScanning analysis(GSA), and then compared the data with quantitative real-time polymerase chain reaction at different time points inperipheral blood (PB) samples of adult B-lineage ALL patients (n=35). The specific polymerase chain reaction (PCR)primers for IGH gene FR-1 and fluorescence-labeled J-primer were used and analyzed by capillary gel electrophoresison a sequencer. The results of this study were compared with the previously reported MRD results obtained by the IGHrearrangements allele-specific oligonucleotide (ASO) -qPCR methods.Results: The total concordance rate was 86.7%, with a P

Published

2023

9. Prevalence and resistance to gastrointestinal parasites in goats: A review

Author

Takalani Judas Mpofu, Khathutshelo Agree Nephawe, and Bohani Mtileni

Subjects

immunoglobulin heavy chain, interferon-gamma resistant, interleukin, major histocompatibility complex, resilience, strongyles, Animal culture, SF1-1100, Veterinary medicine, SF600-1100

Abstract

Gastrointestinal parasitism, particularly nematode infection, is a major health issue affecting goats worldwide, resulting in clinical diseases and productivity loss. Prevalent gastrointestinal parasites (GIPs) affecting goats in South Africa are the Strongyloides papillosus, Eimeria spp., and Strongyles, especially the Haemonchus contortus and Trichostrongylus spp. According to the issues discussed in this paper and by other authors, the prevalence and intensity of various GIPs vary with an animal's location, breed, age, sex, and season. Because GIPs easily develop resistance to chemical treatment, selecting and breeding genetically GIP-resistant animals would be a relatively simple and inexpensive strategy for reducing or eliminating the current reliance on chemotherapy. Potential phenotypic indicators for selecting GIP-resistant goats include parasitological, immunological, and pathological phenotypic markers. Synergistic use of these indicators should be encouraged for a more accurate simplified genotype selection of resistant animals. Genes with Mendelian inheritance, particularly those involved in immunoregulatory mechanisms, have been identified in goats. Exploring this knowledge base to develop cost-effective molecular tools that facilitate enhanced genetic improvement programs is a current challenge. Future statistical and biological models should investigate genetic variations within genomic regions and different candidate genes involved in immunoregulatory mechanisms, as well as the identification of single nucleotide polymorphisms known to affect GIP infection levels.

Published

2022

10. When monoclonal antibodies are not monospecific: Hybridomas frequently express additional functional variable regions

Author

Bradbury, Andrew RM, Trinklein, Nathan D, Thie, Holger, Wilkinson, Ian C, Tandon, Atul K, Anderson, Stephen, Bladen, Catherine L, Jones, Brittany, Aldred, Shelley Force, Bestagno, Marco, Burrone, Oscar, Maynard, Jennifer, Ferrara, Fortunato, Trimmer, James S, Görnemann, Janina, Glanville, Jacob, Wolf, Philipp, Frenzel, Andre, Wong, Julin, Koh, Xin Yu, Eng, Hui-Yan, Lane, David, Lefranc, Marie-Paule, Clark, Mike, and Dübel, Stefan

Subjects

Immunization, Genetics, Vaccine Related, Biotechnology, Animals, Antibodies, Monoclonal, Antibody Specificity, Genes, Immunoglobulin Heavy Chain, Genes, Immunoglobulin Light Chain, Humans, Hybridomas, hybridoma, monoclonal antibodies, specificity, paratope, recombinant antibodies, Immunology, Pharmacology and Pharmaceutical Sciences, Public Health and Health Services

Abstract

Monoclonal antibodies are commonly assumed to be monospecific, but anecdotal studies have reported genetic diversity in antibody heavy chain and light chain genes found within individual hybridomas. As the prevalence of such diversity has never been explored, we analyzed 185 random hybridomas, in a large multicenter dataset. The hybridomas analyzed were not biased towards those with cloning difficulties or known to have additional chains. Of the hybridomas we evaluated, 126 (68.1%) contained no additional productive chains, while the remaining 59 (31.9%) contained one or more additional productive heavy or light chains. The expression of additional chains degraded properties of the antibodies, including specificity, binding signal and/or signal-to-noise ratio, as determined by enzyme-linked immunosorbent assay and immunohistochemistry. The most abundant mRNA transcripts found in a hybridoma cell line did not necessarily encode the antibody chains providing the correct specificity. Consequently, when cloning antibody genes, functional validation of all possible VH and VL combinations is required to identify those with the highest affinity and lowest cross-reactivity. These findings, reflecting the current state of hybridomas used in research, reiterate the importance of using sequence-defined recombinant antibodies for research or diagnostic use.

Published

2018

11. Minimal Residual Disease Detection Using Gene Scanning Analysis, Fluorescent Fragment Analysis, and Capillary Electrophoresis for IgH Rearrangement in Adult B-Lineage Acute Lymphoblastic Leukemia: A Cross-Sectional Study.

Author

Shahkarami, Sepideh, Younesian, Samareh, Rostami, Shahrbano, Kompani, Farzad, Bashash, Davood, Vaezi, Mohammad, and Ghaffari, Seyed Hamidollah

Subjects

*POLYMERASE chain reaction, *LYMPHOBLASTIC leukemia, *ACUTE leukemia, *DENATURING gradient gel electrophoresis, *GENE rearrangement, *CAPILLARY electrophoresis, *CROSS-sectional method, *IMMUNOGLOBULIN heavy chains

Abstract

Objective: Minimal residual disease (MRD) is considered the greatest prognostic factor in acute lymphoblastic leukemia (ALL). MRD is a valuable tool for anticipating impending relapse and treatment response assessment. The objective of the present study was to investigate whether the detection of IgH gene rearrangement using polymerase chain reaction (PCR)-based GeneScan analysis could be a complementary method to monitor MRD along with the quantitative realtime PCR (qPCR). Materials and Methods: In this cross-sectional study, we valued the MRD levels, based on the GeneScanning analysis (GSA), and then compared the data with quantitative real-time polymerase chain reaction at different time points in peripheral blood (PB) samples of adult B-lineage ALL patients (n=35). The specific polymerase chain reaction (PCR) primers for IGH gene FR-1 and fluorescence-labeled J-primer were used and analyzed by capillary gel electrophoresis on a sequencer. The results of this study were compared with the previously reported MRD results obtained by the IGH rearrangements allele-specific oligonucleotide (ASO) -qPCR methods. Results: The total concordance rate was 86.7%, with a P<0.001. MRD results obtained by GSA and ASO-qPCR methods were concordant in all diagnostic samples and samples on the 14th and 28th days of induction therapy. The results of these 2.5 years’ follow-ups demonstrated a significant correlation between the two techniques (r=0.892, P<0.001). Conclusion: It seems that the PCR-based GeneScan analysis of IGH gene rearrangement detection may be a valuable molecular technique to distinguish monoclonality from polyclonality. And also, it may be a precise tool to detect the residual leukemic DNA in the PB follow-up samples of patients. [ABSTRACT FROM AUTHOR]

Published

2023

12. Analysis of IGH allele content in a sample group of rheumatoid arthritis patients demonstrates unrevealed population heterogeneity.

Author

Hardt, Uta, Corcoran, Martin M., Narang, Sanjana, Malmström, Vivianne, Padyukov, Leonid, and Hedestam, Gunilla B. Karlsson

Subjects

RHEUMATOID arthritis, SINGLE nucleotide polymorphisms, IMMUNOGLOBULIN heavy chains, B cell receptors, ALLELES, AGAMMAGLOBULINEMIA

Abstract

Immunoglobulin heavy chain (IGH) germline gene variations influence the B cell receptor repertoire, with resulting biological consequences such as shaping our response to infections and altering disease susceptibilities. However, the lack of information on polymorphism frequencies in the IGH loci at the population level makes association studies challenging. Here, we genotyped a pilot group of 30 individuals with rheumatoid arthritis (RA) to examine IGH allele content and frequencies in this group. Eight novel IGHV alleles and one novel IGHJ allele were identified in the study. 15 cases were haplotypable using heterozygous IGHJ6 or IGHD anchors. One variant, IGHV4-34*01_S0742, was found in three out of 30 cases and included a single nucleotide change resulting in a non-canonical recombination signal sequence (RSS) heptamer. This variant allele, shown by haplotype analysis to be non-expressed, was also found in three out of 30 healthy controls and matched a single nucleotide polymorphism (SNP) described in the 1000 Genomes Project (1KGP) collection with frequencies that varied between population groups. Our finding of previously unreported alleles in a relatively small group of individuals with RA illustrates the need for baseline information about IG allelic frequencies in targeted study groups in preparation for future analysis of these genes in disease association studies. [ABSTRACT FROM AUTHOR]

Published

2023

13. Analysis of IGH allele content in a sample group of rheumatoid arthritis patients demonstrates unrevealed population heterogeneity

Author

Uta Hardt, Martin M. Corcoran, Sanjana Narang, Vivianne Malmström, Leonid Padyukov, and Gunilla B. Karlsson Hedestam

Subjects

immunoglobulin heavy chain, germline gene variation, haplotyping, recombination signal sequence, polymorphism, rheumatoid arthritis, Immunologic diseases. Allergy, RC581-607

Abstract

Immunoglobulin heavy chain (IGH) germline gene variations influence the B cell receptor repertoire, with resulting biological consequences such as shaping our response to infections and altering disease susceptibilities. However, the lack of information on polymorphism frequencies in the IGH loci at the population level makes association studies challenging. Here, we genotyped a pilot group of 30 individuals with rheumatoid arthritis (RA) to examine IGH allele content and frequencies in this group. Eight novel IGHV alleles and one novel IGHJ allele were identified in the study. 15 cases were haplotypable using heterozygous IGHJ6 or IGHD anchors. One variant, IGHV4-34*01_S0742, was found in three out of 30 cases and included a single nucleotide change resulting in a non-canonical recombination signal sequence (RSS) heptamer. This variant allele, shown by haplotype analysis to be non-expressed, was also found in three out of 30 healthy controls and matched a single nucleotide polymorphism (SNP) described in the 1000 Genomes Project (1KGP) collection with frequencies that varied between population groups. Our finding of previously unreported alleles in a relatively small group of individuals with RA illustrates the need for baseline information about IG allelic frequencies in targeted study groups in preparation for future analysis of these genes in disease association studies.

Published

2023

14. B Lymphoblastic Leukemia/Lymphoma With Burkitt-like Morphology and IGH/MYC Rearrangement

Author

Li, Yiting, Gupta, Gunjan, Molofsky, Ari, Xie, Yi, Shihabi, Nader, McCormick, Jane, and Jaffe, Elaine S

Subjects

Pediatric Research Initiative, Pediatric, Orphan Drug, Childhood Leukemia, Cancer, Lymphoma, Hematology, Rare Diseases, Genetics, Pediatric Cancer, Clinical Research, Aetiology, 2.1 Biological and endogenous factors, Adult, Aged, Biomarkers, Tumor, Burkitt Lymphoma, Cell Differentiation, Flow Cytometry, Gene Rearrangement, B-Lymphocyte, Heavy Chain, Genes, Immunoglobulin Heavy Chain, Genetic Predisposition to Disease, Humans, Immunohistochemistry, Immunophenotyping, In Situ Hybridization, Fluorescence, Male, Middle Aged, Phenotype, Precursor B-Cell Lymphoblastic Leukemia-Lymphoma, Proto-Oncogene Proteins c-myc, Treatment Outcome, B lymphoblastic leukemia, lymphoma, MYC rearrangement, Burkitt lymphoma, terminal deoxynucleotidyl transferase, gene (TdT) rearrangement, Clinical Sciences, Pathology

Abstract

Isolated MYC rearrangement without other recurrent genetic abnormalities is rare in B lymphoblastic leukemia/lymphoma (B-ALL/LBL), with most cases reported in pediatric patients. We report 3 adult cases with lymphoblasts showing a precursor B cell immunophenotype, and isolated MYC/IGH translocation. All 3 cases occurred in male patients with initial presentation of diffuse lymphadenopathy. Cases 1 and 2 had B-ALL with significantly increased lymphoblasts in peripheral blood and bone marrow. Case 3, a patient with human immunodeficiency virus infection, had the diagnosis of B-LBL made on a retroperitoneal lymph node biopsy and had no peripheral blood or bone marrow involvement. The leukemic and lymphoma cells in all 3 cases demonstrated Burkitt lymphoma-like morphology with deeply basophilic cytoplasm and numerous cytoplasmic vacuoles. However, all 3 had immature immunophenotypes including expression of terminal deoxynucleotidyl transferase (TdT), absence of BCL6, and dim-to-negative CD45. CD20 was largely negative in 2 of 3 cases. All 3 had confirmed MYC/IGH translocation, but lacked rearrangements of BCL2 or BCL6. EBV was negative by Epstein-Barr virus encoded small RNA in situ hybridization. Treatment protocols varied, including both high-risk ALL-type (protocol 8707) and high-grade lymphoma regimens (hyper-CVAD [cyclophosphamide, vincristine, adriamycin, and dexamethasone]), but no patient achieved continuous complete remission. These cases seem to represent a distinct biological phenomenon, in which a MYC translocation may be acquired at an immature stage of differentiation, thus manifesting features of both B-ALL/LBL and Burkitt lymphoma.

Published

2018

15. Identification of the Antigens Recognised by Colorectal Cancer Patients Using Sera from Patients Who Exhibit a Crohn's-like Lymphoid Reaction.

Author

Boncheva, Viktoriya B., Linnebacher, Michael, Kdimati, Said, Draper, Hannah, Orchard, Laurence, Mills, Ken I., O'Sullivan, Gerald, Tangney, Mark, and Guinn, Barbara-ann

Subjects

*COLORECTAL cancer, *CANCER patients, *ANTIGENS, *IMMUNOGLOBULIN heavy chains

Abstract

A Crohn's-like lymphoid reaction (CLR) is observed in about 15% of colorectal cancer (CRC) patients and is associated with favourable outcomes. To identify the immune targets recognised by CRC CLR patient sera, we immunoscreened a testes cDNA library with sera from three patients. Immunoscreening of the 18 antigens identified by SEREX with sera from normal donors showed that only the heavy chain of IgG3 (IGHG3) and a novel antigen we named UOB-COL-7, were solely recognised by sera from CRC CLR patients. ELISA showed an elevation in IgG3 levels in patients with CRC (p = 0.01). To extend our studies we analysed the expression of our SEREX-identified antigens using the RNA-sequencing dataset (GSE5206). We found that the transcript levels of multiple IGHG probesets were highly significant (p < 0.001) in their association with clinical features of CRC while above median levels of DAPK1 (p = 0.005) and below median levels of GTF2H5 (p = 0.004) and SH3RF2 (p = 0.02) were associated with improved overall survival. Our findings demonstrate the potential of SEREX-identified CRC CLR antigens to act as biomarkers for CRC and provide a rationale for their further characterization and validation. [ABSTRACT FROM AUTHOR]

Published

2022

16. SARS‐CoV‐2 (COVID‐19)‐specific T cell and B cell responses in convalescent rheumatoid arthritis: Monozygotic twins pair case observation.

Author

Arruda, Lucas C. M., Gaballa, Ahmed, Da Silva Rodrigues, Rui, Makower, Bartek, and Uhlin, Michael

Subjects

*B cells, *T cells, *TWINS, *T cell receptors, *IMMUNOGLOBULIN heavy chains, *RHEUMATOID arthritis, *FETOFETAL transfusion

Abstract

Rheumatoid arthritis (RA) patients present higher risk of SARS‐CoV‐2 infection (COVID‐19), and proper management of the disease in this population requires a better understanding of how the immune system controls the virus. We analyzed the T cell and B cell phenotypes, and their repertoire in a pair of monozygotic twins with RA mismatched for COVID‐19 infection. Twin‐ was not infected, while Twin+ was infected and effectively controlled the infection. We found no significant changes on the αβ T cell composition, while γδ T cells and B cells presented considerable expansion of memory population in Twin+ and robust T/B cell responses to several SARS‐CoV‐2 peptides. T cell receptor β/γ‐chain and immunoglobulin heavy chain next‐generation sequencing depicted a remarkable higher diversity in Twin+ compared with Twin‐, despite no significant changes being found in variable/joining family usage. Repertoire overlap analyses showed that, although being identical twins, very few clones were shared between them, indicating that COVID‐19 may lead to deep changes on the immune cell repertoire in RA patients. Altogether, our results indicate that RA patients may develop robust and persistent COVID‐19‐specific T/B cell responses; γδ T cells and B cells may play a key role in the management of COVID‐19 in RA, and the infection may lead to a profound reshaping of immune cell receptor specificities. [ABSTRACT FROM AUTHOR]

Published

2022

17. The Diagnostic and Prognostic Potential of the B-Cell Repertoire in Membranous Nephropathy

Author

Zuhui Su, Yabin Jin, Yu Zhang, Zhanwen Guan, Huishi Li, Xiangping Chen, Chao Xie, Chuling Zhang, Xiaofen Liu, Peixian Li, Peiyi Ye, Lifang Zhang, Yaozhong Kong, and Wei Luo

Subjects

B-cell receptor repertoire, membranous nephropathy, high-throughput sequencing, immunoglobulin heavy chain, biomarkers, Immunologic diseases. Allergy, RC581-607

Abstract

Membranous nephropathy (MN), an autoimmune glomerular disease, is one of the most common causes of nephrotic syndrome in adults. In current clinical practice, the diagnosis is dependent on renal tissue biopsy. A new method for diagnosis and prognosis surveillance is urgently needed for patients. In the present study, we recruited 66 MN patients before any treatment and 11 healthy control (HC) and analyzed multiple aspects of the immunoglobulin heavy chain (IGH) repertoire of these samples using high-throughput sequencing. We found that the abnormalities of CDR-H3 length, hydrophobicity, somatic hypermutation (SHM), and germ line index were progressively more prominent in patients with MN, and the frequency of IGHV3-66 in post-therapy patients was significantly lower than that in pre-therapy patients. Moreover, we found that the IGHV3-38 gene was significantly related to PLA2R, which is the most commonly used biomarker. The most important discovery was that several IGHV, IGHD transcripts, CDR-H3 length, and SHM rate in pre-therapy patients had the potential to predict the therapeutic effect. Our study further demonstrated that the IGH repertoire could be a potential biomarker for prognosis prediction of MN. The landscape of circulating B-lymphocyte repertoires sheds new light on the detection and surveillance of MN.

Published

2021

18. The Diagnostic and Prognostic Potential of the B-Cell Repertoire in Membranous Nephropathy.

Author

Su, Zuhui, Jin, Yabin, Zhang, Yu, Guan, Zhanwen, Li, Huishi, Chen, Xiangping, Xie, Chao, Zhang, Chuling, Liu, Xiaofen, Li, Peixian, Ye, Peiyi, Zhang, Lifang, Kong, Yaozhong, and Luo, Wei

Subjects

IMMUNOGLOBULIN heavy chains, NUCLEOTIDE sequencing, ADULTS, VENTRICULAR septal defects, BIOMARKERS, KIDNEY diseases

Abstract

Membranous nephropathy (MN), an autoimmune glomerular disease, is one of the most common causes of nephrotic syndrome in adults. In current clinical practice, the diagnosis is dependent on renal tissue biopsy. A new method for diagnosis and prognosis surveillance is urgently needed for patients. In the present study, we recruited 66 MN patients before any treatment and 11 healthy control (HC) and analyzed multiple aspects of the immunoglobulin heavy chain (IGH) repertoire of these samples using high-throughput sequencing. We found that the abnormalities of CDR-H3 length, hydrophobicity, somatic hypermutation (SHM), and germ line index were progressively more prominent in patients with MN, and the frequency of IGHV3-66 in post-therapy patients was significantly lower than that in pre-therapy patients. Moreover, we found that the IGHV3-38 gene was significantly related to PLA2R, which is the most commonly used biomarker. The most important discovery was that several IGHV , IGHD transcripts, CDR-H3 length, and SHM rate in pre-therapy patients had the potential to predict the therapeutic effect. Our study further demonstrated that the IGH repertoire could be a potential biomarker for prognosis prediction of MN. The landscape of circulating B-lymphocyte repertoires sheds new light on the detection and surveillance of MN. [ABSTRACT FROM AUTHOR]

Published

2021

19. Development of diagnostic antibodies against immunoglobulin heavy chain variable region for heavy chain amyloidosis (AH amyloidosis).

Author

Nakagawa, Mayuko, Yazaki, Masahide, Kametani, Fuyuki, Katoh, Nagaaki, Yoshinaga, Tsuneaki, Higuchi, Keiichi, and Sekijima, Yoshiki

Subjects

*IMMUNOGLOBULIN heavy chains, *AMYLOIDOSIS, *IMMUNOGLOBULINS, *MOLECULAR weights

Abstract

It is difficult to diagnose immunoglobulin heavy chain amyloidosis (AH amyloidosis) without proteomic analysis due to no useful diagnostic antibodies. The aim of this study was to develop diagnostic antibodies available to immunohistochemistry and immunoblotting. Two rabbit anti‐heavy chain variable region antibodies were generated and evaluated in immunohistochemical studies performed on 11 AH amyloidosis patients and 64 patients with other systemic amyloidoses. Additionally, immunoblotting was performed using extracted amyloid protein from one patient and serum samples from two patients with AH amyloidosis. Immunohistochemical analysis generated a positive outcome in 10 of 11 AH amyloidosis patients (sensitivity 90.9%). While positive staining was also observed in 9 of 64 non‐AH amyloidosis patients (specificity 85.9%), substitution of the blocking agent reversed the positive reactivity in 5 of 9 patients. Amyloid protein band was clearly detected via immunoblotting analysis, and protein bands with similar molecular weights of amyloid protein were observed in serum samples from patients with AH amyloidosis. The two antibodies may represent a powerful diagnostic tool for AH amyloidosis. In addition, our data revealed the existence of amyloidogenic variable region fragments in the serum of patients, suggesting their potential as diagnostic markers for AH amyloidosis. [ABSTRACT FROM AUTHOR]

Published

2021

20. Correlations in Somatic Hypermutation Between Sites in IGHV Genes Can Be Explained by Interactions Between AID and/or Polη Hotspots

Author

Artem Krantsevich, Catherine Tang, and Thomas MacCarthy

Subjects

B cell receptor, activation-induced deaminase, computational immunology, immunoglobulin heavy chain, somatic hypermutation, overlapping hotspots, Immunologic diseases. Allergy, RC581-607

Abstract

The somatic hypermutation (SHM) of Immunoglobulin (Ig) genes is a key process during antibody affinity maturation in B cells. The mutagenic enzyme activation induced deaminase (AID) is required for SHM and has a preference for WRC hotspots in DNA. Error-prone repair mechanisms acting downstream of AID introduce further mutations, including DNA polymerase eta (Polη), part of the non-canonical mismatch repair pathway (ncMMR), which preferentially generates mutations at WA hotspots. Previously proposed mechanistic models lead to a variety of predictions concerning interactions between hotspots, for example, how mutations in one hotspot will affect another hotspot. Using a large, high-quality, Ig repertoire sequencing dataset, we evaluated pairwise correlations between mutations site-by-site using an unbiased measure similar to mutual information which we termed “mutational association” (MA). Interactions are dominated by relatively strong correlations between nearby sites (short-range MAs), which can be almost entirely explained by interactions between overlapping hotspots for AID and/or Polη. We also found relatively weak dependencies between almost all sites throughout each gene (longer-range MAs), although these arise mostly as a statistical consequence of high pairwise mutation frequencies. The dominant short-range interactions are also highest within the most highly mutating IGHV sub-regions, such as the complementarity determining regions (CDRs), where there is a high hotspot density. Our results suggest that the hotspot preferences for AID and Polη have themselves evolved to allow for greater interactions between AID and/or Polη induced mutations.

Published

2021

21. Evaluation of Somatic Hypermutation Status in Chronic Lymphocytic Leukemia (CLL) in the Era of Next Generation Sequencing

Author

Sanjeev Kumar Gupta, David S. Viswanatha, and Keyur P. Patel

Subjects

CLL, somatic hypermutation, NGS, clonality, immunoglobulin heavy chain, Biology (General), QH301-705.5

Abstract

Somatic hypermutation (SHM) status provides an important prognostic indicator for chronic lymphocytic leukemia (CLL), a very common type of mature B-cell leukemia. Owing to the adverse prognosis associated with an unmutated immunoglobulin heavy chain variable (IGHV) status, SHM testing is performed as a standard of care in CLL. Conventionally, SHM testing has been performed using labor intensive and primarily analog Sanger sequencing method following PCR amplification of the clonal immunoglobulin heavy chain gene rearrangements in CLL cells. In comparison, recent availability of next generation sequencing (NGS) allows more versatile detection and direct identification of clonal immunoglobulin gene rearrangements in neoplastic B-cell populations. The ability to identify specific clonal IGHV signature(s) in both baseline (diagnostic) and post-treatment settings enables unique clinical applications of NGS such as determination of SHM status, minimal residual disease (MRD) monitoring, clonal heterogeneity and B cell receptor IG stereotypy. We provide a review of current practices and recommendations for SHM determination using NGS including examples of difficult cases.

Published

2020

22. AID Overlapping and Polη Hotspots Are Key Features of Evolutionary Variation Within the Human Antibody Heavy Chain (IGHV) Genes

Author

Catherine Tang, Davide Bagnara, Nicholas Chiorazzi, Matthew D. Scharff, and Thomas MacCarthy

Subjects

somatic hypermutation (SHM), activation induced deaminase (AID), immunoglobulin heavy chain, computational immunology, B cell receptor (BCR), dimensionality reduction, Immunologic diseases. Allergy, RC581-607

Abstract

Somatic hypermutation (SHM) of the immunoglobulin variable (IgV) loci is a key process in antibody affinity maturation. The enzyme activation-induced deaminase (AID), initiates SHM by creating C → U mismatches on single-stranded DNA (ssDNA). AID has preferential hotspot motif targets in the context of WRC/GYW (W = A/T, R = A/G, Y = C/T) and particularly at WGCW overlapping hotspots where hotspots appear opposite each other on both strands. Subsequent recruitment of the low-fidelity DNA repair enzyme, Polymerase eta (Polη), during mismatch repair, creates additional mutations at WA/TW sites. Although there are more than 50 functional immunoglobulin heavy chain variable (IGHV) segments in humans, the fundamental differences between these genes and their ability to respond to all possible foreign antigens is still poorly understood. To better understand this, we generated profiles of WGCW hotspots in each of the human IGHV genes and found the expected high frequency in complementarity determining regions (CDRs) that encode the antigen binding sites but also an unexpectedly high frequency of WGCW in certain framework (FW) sub-regions. Principal Components Analysis (PCA) of these overlapping AID hotspot profiles revealed that one major difference between IGHV families is the presence or absence of WGCW in a sub-region of FW3 sometimes referred to as “CDR4.” Further differences between members of each family (e.g., IGHV1) are primarily determined by their WGCW densities in CDR1. We previously suggested that the co-localization of AID overlapping and Polη hotspots was associated with high mutability of certain IGHV sub-regions, such as the CDRs. To evaluate the importance of this feature, we extended the WGCW profiles, combining them with local densities of Polη (WA) hotspots, thus describing the co-localization of both types of hotspots across all IGHV genes. We also verified that co-localization is associated with higher mutability. PCA of the co-localization profiles showed CDR1 and CDR2 as being the main contributors to variance among IGHV genes, consistent with the importance of these sub-regions in antigen binding. Our results suggest that AID overlapping (WGCW) hotspots alone or in conjunction with Polη (WA/TW) hotspots are key features of evolutionary variation between IGHV genes.

Published

2020

23. Correlations in Somatic Hypermutation Between Sites in IGHV Genes Can Be Explained by Interactions Between AID and/or Polη Hotspots.

Author

Krantsevich, Artem, Tang, Catherine, and MacCarthy, Thomas

Subjects

ENZYME activation, DNA polymerases, GENES, B cell receptors, B cells, DNA mismatch repair, IMMUNOGLOBULIN class switching

Abstract

The somatic hypermutation (SHM) of Immunoglobulin (Ig) genes is a key process during antibody affinity maturation in B cells. The mutagenic enzyme activation induced deaminase (AID) is required for SHM and has a preference for WR C hotspots in DNA. Error-prone repair mechanisms acting downstream of AID introduce further mutations, including DNA polymerase eta (Polη), part of the non-canonical mismatch repair pathway (ncMMR), which preferentially generates mutations at W A hotspots. Previously proposed mechanistic models lead to a variety of predictions concerning interactions between hotspots, for example, how mutations in one hotspot will affect another hotspot. Using a large, high-quality, Ig repertoire sequencing dataset, we evaluated pairwise correlations between mutations site-by-site using an unbiased measure similar to mutual information which we termed "mutational association" (MA). Interactions are dominated by relatively strong correlations between nearby sites (short-range MAs), which can be almost entirely explained by interactions between overlapping hotspots for AID and/or Polη. We also found relatively weak dependencies between almost all sites throughout each gene (longer-range MAs), although these arise mostly as a statistical consequence of high pairwise mutation frequencies. The dominant short-range interactions are also highest within the most highly mutating IGHV sub-regions, such as the complementarity determining regions (CDRs), where there is a high hotspot density. Our results suggest that the hotspot preferences for AID and Polη have themselves evolved to allow for greater interactions between AID and/or Polη induced mutations. [ABSTRACT FROM AUTHOR]

Published

2021

24. Chapter Four - Panorama of stepwise involvement of the IgH 3' regulatory region in murine B cells.

Author

Bruzeau, Charlotte, Moreau, Jeanne, Noir, Sandrine Le, and Pinaud, Eric

Subjects

B cells, B cell receptors, IMMUNOGLOBULIN class switching, IMMUNOGLOBULIN heavy chains, PLASMA cells

Abstract

Among the multiple events leading to immunoglobulin (Ig) expression in B cells, stepwise activation of the Ig heavy chain locus (IgH) is of critical importance. Transcription regulation of the complex IgH locus has always been an interesting viewpoint to unravel the multiple and complex events required for IgH expression. First, regulatory germline transcripts (GLT) assist DNA remodeling events such as VDJ recombination, class switch recombination (CSR) and somatic hypermutation (SHM). Second, productive spliced transcripts restrict heavy chain protein expression associated either with the surface receptor of developing B cells or secreted in large amounts in plasma cells. One main transcriptional regulator for IgH lies at its 3' extremity and includes both a set of enhancers grouped in a large 3' regulatory region (3'RR) and a cluster of 3'CTCF-binding elements (3'CBEs). In this focused review, we will preferentially refer to evidence reported for the murine endogenous IgH locus, whether it is wt or carries deletions or insertions within the IgH 3' boundary and associated regulatory region. [ABSTRACT FROM AUTHOR]

Published

2021

25. AID Overlapping and Polη Hotspots Are Key Features of Evolutionary Variation Within the Human Antibody Heavy Chain (IGHV) Genes.

Author

Tang, Catherine, Bagnara, Davide, Chiorazzi, Nicholas, Scharff, Matthew D., and MacCarthy, Thomas

Subjects

DNA mismatch repair, DNA ligases, IMMUNOGLOBULIN heavy chains, SINGLE-stranded DNA, BINDING sites, PRINCIPAL components analysis

Abstract

Somatic hypermutation (SHM) of the immunoglobulin variable (IgV) loci is a key process in antibody affinity maturation. The enzyme activation-induced deaminase (AID), initiates SHM by creating C → U mismatches on single-stranded DNA (ssDNA). AID has preferential hotspot motif targets in the context of WR C / G YW (W = A/T, R = A/G, Y = C/T) and particularly at W GC W overlapping hotspots where hotspots appear opposite each other on both strands. Subsequent recruitment of the low-fidelity DNA repair enzyme, Polymerase eta (Polη), during mismatch repair, creates additional mutations at W A / T W sites. Although there are more than 50 functional immunoglobulin heavy chain variable (IGHV) segments in humans, the fundamental differences between these genes and their ability to respond to all possible foreign antigens is still poorly understood. To better understand this, we generated profiles of WGCW hotspots in each of the human IGHV genes and found the expected high frequency in complementarity determining regions (CDRs) that encode the antigen binding sites but also an unexpectedly high frequency of WGCW in certain framework (FW) sub-regions. Principal Components Analysis (PCA) of these overlapping AID hotspot profiles revealed that one major difference between IGHV families is the presence or absence of WGCW in a sub-region of FW3 sometimes referred to as "CDR4." Further differences between members of each family (e.g., IGHV1) are primarily determined by their WGCW densities in CDR1. We previously suggested that the co-localization of AID overlapping and Polη hotspots was associated with high mutability of certain IGHV sub-regions, such as the CDRs. To evaluate the importance of this feature, we extended the WGCW profiles, combining them with local densities of Polη (WA) hotspots, thus describing the co-localization of both types of hotspots across all IGHV genes. We also verified that co-localization is associated with higher mutability. PCA of the co-localization profiles showed CDR1 and CDR2 as being the main contributors to variance among IGHV genes, consistent with the importance of these sub-regions in antigen binding. Our results suggest that AID overlapping (WGCW) hotspots alone or in conjunction with Polη (WA/TW) hotspots are key features of evolutionary variation between IGHV genes. [ABSTRACT FROM AUTHOR]

Published

2020

26. Unveiling the Diversity of Immunoglobulin Heavy Constant Gamma (IGHG) Gene Segments in Brazilian Populations Reveals 28 Novel Alleles and Evidence of Gene Conversion and Natural Selection

Author

Verónica Calonga-Solís, Danielle Malheiros, Marcia Holsbach Beltrame, Luciana de Brito Vargas, Renata Montoro Dourado, Hellen Caroline Issler, Roseli Wassem, Maria Luiza Petzl-Erler, and Danillo G. Augusto

Subjects

IGHG genes, immunoglobulin heavy chain, molecular characterization, genetic diversity, populations, DNA sequencing, Immunologic diseases. Allergy, RC581-607

Abstract

Even though immunoglobulins are critical for immune responses and human survival, the diversity of the immunoglobulin heavy chain gene (IGH) is poorly known and mostly characterized only by serological methods. Moreover, this genomic region is not well-covered in genomic databases and genome-wide association studies due to particularities that impose technical difficulties for its analysis. Therefore, the IGH gene has never been systematically sequenced across populations. Here, we deliver an unprecedented and comprehensive characterization of the diversity of the IGHG1, IGHG2, and IGHG3 gene segments, which encode the constant region of the most abundant circulating immunoglobulins: IgG1, IgG2, and IgG3, respectively. We used Sanger sequencing to analyze 357 individuals from seven different Brazilian populations, including five Amerindian, one Japanese-descendant and one Euro-descendant population samples. We discovered 28 novel IGHG alleles and provided evidence that some of them may have been originated by gene conversion between common alleles of different gene segments. The rate of synonymous substitutions was significantly higher than the rate of the non-synonymous substitutions for IGHG1 and IGHG2 (p = 0.01 and 0.03, respectively), consistent with purifying selection. Fay and Wu's test showed significant negative values for most populations (p < 0.001), which indicates that positive selection in an adjacent position may be shaping IGHG variation by hitchhiking of variants in the vicinity, possibly the regions that encode the Ig variable regions. This study shows that the variation in the IGH gene is largely underestimated. Therefore, exploring its nucleotide diversity in populations may provide valuable information for comprehension of its evolution, its impact on diseases and vaccine research.

Published

2019

27. Unveiling the Diversity of Immunoglobulin Heavy Constant Gamma (IGHG) Gene Segments in Brazilian Populations Reveals 28 Novel Alleles and Evidence of Gene Conversion and Natural Selection.

Author

Calonga-Solís, Verónica, Malheiros, Danielle, Beltrame, Marcia Holsbach, Vargas, Luciana de Brito, Dourado, Renata Montoro, Issler, Hellen Caroline, Wassem, Roseli, Petzl-Erler, Maria Luiza, and Augusto, Danillo G.

Subjects

IMMUNOGLOBULINS, GENE conversion, ALLELES, NATURAL selection, NUCLEOTIDE sequencing

Abstract

Even though immunoglobulins are critical for immune responses and human survival, the diversity of the immunoglobulin heavy chain gene (IGH) is poorly known and mostly characterized only by serological methods. Moreover, this genomic region is not well-covered in genomic databases and genome-wide association studies due to particularities that impose technical difficulties for its analysis. Therefore, the IGH gene has never been systematically sequenced across populations. Here, we deliver an unprecedented and comprehensive characterization of the diversity of the IGHG1, IGHG2 , and IGHG3 gene segments, which encode the constant region of the most abundant circulating immunoglobulins: IgG1, IgG2, and IgG3, respectively. We used Sanger sequencing to analyze 357 individuals from seven different Brazilian populations, including five Amerindian, one Japanese-descendant and one Euro-descendant population samples. We discovered 28 novel IGHG alleles and provided evidence that some of them may have been originated by gene conversion between common alleles of different gene segments. The rate of synonymous substitutions was significantly higher than the rate of the non-synonymous substitutions for IGHG1 and IGHG2 (p = 0.01 and 0.03, respectively), consistent with purifying selection. Fay and Wu's test showed significant negative values for most populations (p < 0.001), which indicates that positive selection in an adjacent position may be shaping IGHG variation by hitchhiking of variants in the vicinity, possibly the regions that encode the Ig variable regions. This study shows that the variation in the IGH gene is largely underestimated. Therefore, exploring its nucleotide diversity in populations may provide valuable information for comprehension of its evolution, its impact on diseases and vaccine research. [ABSTRACT FROM AUTHOR]

Published

2019

28. Genetic analysis of Diffuse Large B‐cell Lymphoma occurring in cases with antecedent Waldenström Macroglobulinaemia reveals different patterns of clonal evolution.

Author

Talaulikar, Dipti, Biscoe, Amber, Lim, Jun H., Gibson, John, Arthur, Christopher, Mackinlay, Naomi, Saxena, Kartik, Cheng, Yuen Y., and Chen, Vivien M.

Subjects

*WALDENSTROM'S macroglobulinemia, *LYMPHOMAS, *B cell receptors, *IMMUNOGLOBULIN heavy chains

Abstract

The article talks on the treatment therapy of Waldenstr€om Macroglobulinaemia (WM) . Topics discussed include WM is a rare indolent B-cell malignancy characterized by IgM paraprotein and bone marrow (BM) infiltration by clonal lymphocytes, mentions the Diffusion of large B-cell lymphoma (DLBCL), that may result in histological transformation of the WM clone, and highlights the importance of identifying pathways for transformation as opposed to de novo second B-cell lymphomas.

Published

2019

29. High-risk subtypes of chronic lymphocytic leukemia are detectable as early as 16 years prior to diagnosis

Author

Kolijn, Martijn, Saberi Hosnijeh, Fatemeh, Spath, Florentin, Hengeveld, P., Andreas, Agathangelidis, Saleh, Manal, Casabonne, Delphine, Benavente, Yolanda, Jerkeman, Mats, Aguado, Antonio, Barricante, Aurelio, Besson, Caroline M, Sanchez, Maria-Jose, Chirlaque, Maria Dolores, Masala, Giovanna, Sacerdote, Carlotta, Grioni, Sara, Schulze, M.B., Nieters, Alexandra, Engelfriet, Peter M, Hultdin, Magnus, McKay, J., Vermeulen, Roel, Langerak, Anton W, IRAS OH Epidemiology Chemical Agents, IRAS OH Epidemiology Chemical Agents, and Immunology

Subjects

Lymphocytosis, Chronic lymphocytic leukemia, Immunology, Somatic hypermutation, Receptors, Antigen, B-Cell, Biochemistry, immune system diseases, hemic and lymphatic diseases, Medicine, Humans, Hematologi, Gene, Aged, Cancer och onkologi, B-Lymphocytes, business.industry, Repertoire, breakpoint cluster region, Cell Biology, Hematology, medicine.disease, Leukemia, Lymphocytic, Chronic, B-Cell, Cancer and Oncology, Monoclonal, Immunoglobulin heavy chain, medicine.symptom, business, Immunoglobulin Heavy Chains

Abstract

Chronic lymphocytic leukemia (CLL) is preceded by monoclonal B-cell lymphocytosis (MBL), a CLL precursor state with a prevalence of up to 12% in aged individuals; however, the duration of MBL and the mechanisms of its evolution to CLL remain largely unknown. In this study, we sequenced the B-cell receptor (BcR) immunoglobulin heavy chain (IGH) gene repertoire of 124 patients with CLL and 118 matched controls in blood samples taken up to 22 years prior to diagnosis. Significant skewing in the BcR IGH gene repertoire was detected in the majority of patients, even before the occurrence of lymphocytosis and irrespective of the clonotypic IGH variable gene somatic hypermutation status. Furthermore, we identified dominant clonotypes belonging to major stereotyped subsets associated with poor prognosis up to 16 years before diagnosis in 14 patients with CLL. In 22 patients with longitudinal samples, the skewing of the BcR IGH gene repertoire increased significantly over time to diagnosis or remained stable at high levels. For 14 of 16 patients with available samples at diagnosis, the CLL clonotype was already present in the prediagnostic samples. Overall, our data indicate that the preclinical phase of CLL could be longer than previously thought, even in adverse-prognostic cases.

Published

2022

30. Histopathologic, immunophenotypic, and mutational landscape of follicular lymphomas with plasmacytic differentiation

Author

Svetlana A. Yatsenko, Sarah E. Gibson, Yen-Chun Liu, Steven H. Swerdlow, and Nicholas Barasch

Subjects

Pathology, medicine.medical_specialty, EZH2, Biology, medicine.disease, Marginal zone, BCL6, Pathology and Forensic Medicine, immune system diseases, hemic and lymphatic diseases, Cancer genetics, Follicular phase, medicine, Centroblasts, Immunoglobulin heavy chain, B-cell lymphoma

Abstract

Follicular lymphomas with plasmacytic differentiation (FL-PCD) include two major subtypes: one with predominantly interfollicular PCD that usually harbors a BCL2 rearrangement (BCL2-R), and a second that has predominantly intrafollicular PCD and the frequent absence of a BCL2-R. It is proposed that these latter cases share some features with marginal zone lymphomas (MZL). To further explore this hypothesis in an expanded cohort of FL-PCD, a clinicopathologic investigation of 25 such cases was undertaken including an analysis of their mutational landscape. The 10 interfollicular FL-PCDs exhibited typical intrafollicular centrocytes/centroblasts (90%), CD10 expression (90%), full PCD including expression of CD138 by the plasma cells (PC) (100%), and PCs with class-switched immunoglobulin heavy chains (70%). These cases were BCL2-R positive (100%), BCL6-R positive in 30%, lacked extra BCL2 copies, and only 22% had extra copies of BCL6. Similar to classic FLs, 80% of interfollicular FL-PCDs harbored mutations in epigenetic regulators KMT2D (70%), CREBBP (40%), and/or EZH2 (30%). In contrast, only 45% of 11 intrafollicular FL-PCDs demonstrated typical intrafollicular centrocytes/centroblasts, 55% were CD10(-), 80% contained IgM+ PCs, and only 27% harbored BCL2-Rs. BCL6-Rs were identified in 27% of intrafollicular FL-PCD, while 60% showed extra copies of BCL2 and 50% extra copies of BCL6, consistent with complete or partial trisomies of chromosomes 18 and 3, respectively. Only 54% of intrafollicular FL-PCDs showed mutations in epigenetic regulators. Both subtypes showed mutational differences compared to classic FL, but only the interfollicular subtype showed differences from what is reported for nodal MZL. Four additional cases showed mixed intra- and interfollicular PCD. These results suggest that FL-PCD has some distinctive features and supports the existence of two major subtypes. The interfollicular PCD subtype shares many features with classic FL. The intrafollicular FL-PCDs are more heterogeneous, have differences from classic FL, and have a greater morphologic, immunophenotypic, and genetic overlap with MZL.

Published

2022

31. Molecular Biology and Classification of Multiple Myeloma

Author

Dmoszyńska, Anna, Grząśko, Norbert, Witt, Michal, editor, Dawidowska, Malgorzata, editor, and Szczepanski, Tomasz, editor

Published

2012

32. Pulmonary Nodular Lymphoid Hyperplasia Evaluated with Bronchoalveolar Lavage Fluid Findings: A Case Report and Review of the Literature on Japanese Patients

Author

Sakiko Moriyama, Takashi Kido, Noriho Sakamoto, Mai Fuchigami, Takatomo Tokito, Daisuke Okuno, Takuto Miyamura, Shota Nakashima, Atsuko Hara, Hiroshi Ishimoto, Yoshitaka Imaizumi, Kazuto Tsuruda, Katsunori Yanagihara, Junya Fukuoka, and Hiroshi Mukae

Subjects

Adult, Lung Diseases, Hyperplasia, East Asian People, immunoglobulin heavy chain, General Medicine, Lymphoma, B-Cell, Marginal Zone, Internal Medicine, Humans, Female, gene translocation, Bronchoalveolar Lavage Fluid, mucosaassociated lymphoid tissue lymphoma, pulmonary nodular lymphoid hyperplasia

Abstract

Pulmonary nodular lymphoid hyperplasia (PNLH) is a very rare disease, and it is difficult to diagnose PNLH and distinguish it from mucosa-associated lymphoid tissue (MALT) lymphoma. In addition, information on bronchoalveolar lavage fluid (BALF) analyses is lacking. We herein report a 36-year-old Japanese woman diagnosed with PLNH by a surgical biopsy and analysis of BALF. The BALF showed an increase in B-cell marker-positive lymphocytes, normal patterns of B-cell clonality, mucosa-associated lymphoid tissue 1 gene, and immunoglobulin heavy chain at 14q32 translocations. We also reviewed Japanese cases of PNLH described in Japanese or English to explore the characteristics of such cases., Internal Medicine, 62(1), pp.95-102; 2023

Published

2023

33. A clinical perspective on immunoglobulin heavy chain clonal heterogeneity in B cell acute lymphoblastic leukemia.

Author

Fries, Carol and Burack, W. Richard

Subjects

*IMMUNOGLOBULIN heavy chains, *B cells, *LYMPHOBLASTIC leukemia, *BIOMARKERS, *GENE rearrangement

Abstract

Highlights • Abundant intra-clonal heterogeneity exists within acute lymphoblastic leukemia. • Intra-clonal variation complicates the interpretation of leukemia detection assays. • Sequencing-based methods may enhance minimal residual disease detection sensitivity. Abstract B cell acute lymphoblastic leukemia (B ALL) is a genetically heterogeneous neoplasm often demonstrating extensive subclone diversity within each patient's disease. The immunoglobulin heavy chain (IGH) locus is a marker of clonal variation in B ALL due to its intrinsic role in B lymphocyte development and its diverse Vh(D)Jh rearrangement patterns. B ALL IGH evolution may contribute to limitations in minimal residual disease (MRD) monitoring methods. Evolving technologies for IGH high-throughput sequencing (HTS) have demonstrated MRD detection as sensitive as 1 cell in 1,000,000. These methods may enhance the surveillance of B ALL in the setting of extensive subclone evolution and provide opportunities for detection and intervention before the onset of relapse. However, HTS MRD methods will need to be evaluated in the context of clinical trials in order to gain further insights about the clinical relevance of such sensitive B ALL MRD detection. [ABSTRACT FROM AUTHOR]

Published

2018

34. Immunoglobulin heavy chain variable region analysis in dairy goats.

Author

Du, Lijuan, Wang, Shuhui, Zhu, Yanjiao, Zhao, Haidong, Basit, Abdul, Yu, Xiaohui, Li, Qingwang, and Sun, Xiuzhu

Subjects

*IMMUNOGLOBULIN heavy chains, *GOATS, *IMMUNOGLOBULIN H, *ANTISENSE DNA, *SOMATIC mutation

Abstract

Highlights • A brief germline genome organization of goat immunoglobulin heavy chain variable region was revealed. • Ten goat IgH variable genes were found, and the potentially functional segments were belong to a same gene family. • Potentially functional genes (three D H and two J H ) encoded the majority IgH variable region repertoire in goat. • VDJ recombination played a limited role in goat IgH variable repertoire diversification, and SHM is the major goat IgH diversity mechanism. Abstract Based on the goat genome database, we have annotated the genomic organization of the goat immunoglobulin heavy chain variable region. The goat IgH locus is present on seven genome scaffolds, and contains ten V H , three D H and six J H segments. After the exclusion of three shorter segments, the V H genes were divided into two gene families based on sequence similarity. By analyzing the IgH cDNA sequences, we further identified that V H 2 (54.2%), D H 1 (61.7%) and J H 1 (60.5%) segments were most frequently utilized in the expression of the immunoglobulin variable region, and that point mutations introduced by somatic hypermutation were the major mutation present in these expressed variable region. Compared with human and horses, D H -D H fusion occurred at a higher frequency in goat V(D)J recombination. These results provided variable insights into goat immunoglobulin heavy chain variable region genome loci and repertoire diversity. [ABSTRACT FROM AUTHOR]

Published

2018

35. PCR-based clonality analysis of antigen receptor gene rearrangements in canine cutaneous plasmacytoma.

Author

Takanosu, M., Okada, K., and Kagawa, Y.

Subjects

*CUSPIDS, *PLASMACYTOMA, *ANTIGEN receptors

Abstract

Highlights • The sensitivity of PCR-based clonality analysis of IGH gene rearrangements in canine cutaneous plasmacytoma was determined. • Plasmacytomas, diffuse large B cell lymphomas (DLBCLs) and non-lymphoma lymph nodes (LNs) were studied. • IGH clonality was detected in 0–34.5% of plasmacytomas and 17.4–78.3% of DLBCLs. • IGH clonality was detected in only one LN without lymphoma with two out of the seven oligonucleotide primers. • The low frequency of detection of IGH clonality in canine plasmacytomas may reflect variable region somatic hypermutation. Abstract Plasmacytomas are discrete, B cell-derived, round cell tumours that sometimes are difficult to distinguish from canine cutaneous histiocytomas or T cell lymphosarcomas (lymphomas). Diagnosis of plasmacytomas relies on morphological observations and immunohistochemistry for multiple myeloma oncogene-1 (MUM-1) and cluster of differentiation 3 (CD3). Clonality testing often is used as an adjunct diagnostic tool to examine lymphoproliferative diseases. In this study, the sensitivity of PCR-based clonality analysis of antigen receptor gene rearrangements in canine cutaneous plasmacytomas was determined. Formalin-fixed paraffin-embedded sections of 29 canine plasmacytomas, 23 diffuse large B cell lymphomas (DLBCLs) and 23 lymph nodes without lymphoma were used for clonality analysis. New oligonucleotide primers for the framework (FR)2 and FR3 regions of the immunoglobulin heavy chain (IGH) V gene subgroup 3 were designed and used with previously reported FR3 primers. Although plasma cells are of B cell lineage, the detected frequency of IGH clonality in plasmacytoma was 0–34.5% with the seven primers used, whereas in DLBCLs it was 8.7–78.3%. In 23 lymph nodes without lymphoma, IGH clonality was detected in only one case with two out of the seven primers used. Sequence analysis of PCR products from plasmacytomas revealed mismatches in the annealing region of the FR3 primers. The sensitivity of detecting IGH clonality in canine plasmacytomas was lower than in DLBCLs. The low detection rate of IGH clonality in canine plasmacytoma may be due to somatic hypermutation of the variable region. [ABSTRACT FROM AUTHOR]

Published

2018

36. Monitoring immunoglobulin heavy chain and T-cell receptor gene rearrangement in cfDNA as minimal residual disease detection for patients with acute myeloid leukemia.

Author

Zhong, Ling, ChEN, Jiao, Huang, Xiaobing, Li, Yanxing, and Jiang, Tao

Subjects

*T cells, *IMMUNOGLOBULIN heavy chains, *ACUTE myeloid leukemia, *CANCER chemotherapy, *POLYMERASE chain reaction

Abstract

The present study aimed to examine whether monoclonal immunoglobulin heavy chain (IGH) or T-cell receptor (TCR) gene rearrangement in cell-free DNA (cfDNA) may be used for minimal residual disease (MRD) monitoring in patients with acute myeloid leukemia (AML). Monoclonal IGH and TCR rearrangement in cfDNA were monitored in patients with AML. A total of 94 (40%) patients had monoclonal IGH or TCR rearrangements in cfDNA at diagnosis; 84% of these patients (79 cases) achieved complete remission following 1-3 courses of induction chemotherapy. Among these cases, 89.9% were negative for monoclonal IGH or TCR rearrangement in cfDNA following consolidation chemotherapies. A total of 8 patients with consistently positive monoclonal IGH or TCR rearrangement in cfDNA relapsed within 6-10 months. During follow up, 39 patients demonstrated positive monoclonal IGH or TCR rearrangement in cfDNA and relapsed. Recurrence of monoclonal IGH or TCR rearrangement in cfDNA was observed 1-3 months earlier than bone marrow relapse and 11 patients with solitary extramedullary relapse demonstrated positive monoclonal IGH or TCR rearrangement recurrence in cfDNA. In conclusion, the detection of monoclonal IGH and TCR rearrangement in cfDNA may represent a useful tool for MRD monitoring in patients with AML. [ABSTRACT FROM AUTHOR]

Published

2018

37. Chapter Three - RAG Chromatin Scanning During V(D)J Recombination and Chromatin Loop Extrusion are Related Processes.

Author

Lin, Sherry G., Zhaoqing Ba, Alt, Frederick W., and Yu Zhang

Subjects

IMMUNOLOGY periodicals, CHROMATIN, IMMUNE system, T cells

Abstract

An effective adaptive immune system depends on the ability of developing B and T cells to generate diverse immunoglobulin (Ig) and T cell receptor repertoires, respectively. Such diversity is achieved through a programmed somatic recombination process whereby germline V, D, and J segments of antigen receptor loci are assembled to form the variable region V(D)J exons of Ig and TCRs. Studies of this process, termed V(D)J recombination, have provided key insights into our understanding of a variety of general gene regulatory and DNA repair processes over the last several decades. V(D)J recombination is initiated by the RAG endonuclease which generates DNA double-stranded breaks at the borders of V, D, and J segments. In this review, we cover recent work that has elucidated RAG structure and work that revealed that RAG has a novel chromatin scanning activity, likely mediated by chromatin loop extrusion, that contributes to its ability to locate V, D, J gene segment substrates within large chromosomal loop domains bounded by CTCF-binding elements (CBEs). This latter function, coupled with the role CBE-based chromatin loop domains and subdomains within them play in focusing V(D)J recombination activity within antigen receptor loci, provide mechanistic explanations for long-standing questions regarding V(D)J segment usage diversification and in limiting potentially deleterious off-target RAG-initiated recombination events genome-wide. This review will focus mainly on studies of the mouse Ig heavy chain locus, but the principles described also apply to other Ig loci and to TCR loci in mice and humans. [ABSTRACT FROM AUTHOR]

Published

2018

38. In silico analysis identifies CRISP3 as a potential peripheral blood biomarker for multiple myeloma: From data modeling to validation with RT-PCR.

Author

Leng, Dong, Miao, Ran, Huang, Xiaoxi, and Wang, Ying

Subjects

*MULTIPLE myeloma, *CRISPRS, *GENE expression, *IMMUNOGLOBULIN heavy chains, *BIOINDICATORS, *GLYCOPROTEINS, *GENETICS

Abstract

Octamer-binding protein 2 (Oct2) binds to the ATGCAAAT octamer on the IgH enhancer and stimulates IgH expression in human multiple myeloma (MM). Cysteine-rich secreted protein 3 (CRISP3) possesses the ATGCAAAT sequence and thus is activated by Oct2 in mouse B cells, suggesting that CRISP3 may be activated in and be a potential biomarker for MM. The present study involved a meta-analysis of the gene expression profiling data of human MM peripheral blood. Significantly expressed genes were analyzed on merged super array microarray data and selected sample data with significantly expressed genes were additionally analyzed by principal component analysis and Bayesian probit regression. CRISP3, Oct2, Apha-1B-glycoprotein (A1GB) and Cyclin D2 (CCND2) were validated in clinical MM peripheral blood samples using reverse transcription quantitative polymerase chain reaction. In the gene expression profiling data, CRISP3 was significantly upregulated and had certain proportions on the discriminated principal component of significantly expressed gene sample data. RT-qPCR analysis revealed CRISP3 was significantly upregulated in MM. Therefore, CRISP3 is a potential peripheral blood biomarker for MM. [ABSTRACT FROM AUTHOR]

Published

2018

39. Heterogeneous origin of IgE in atopic dermatitis and psoriasis revealed by B cell receptor repertoire analysis

Author

Wei Li, Ronghui Zhu, Xiao Liu, Xu Yao, Jinghua Wu, Jing Xu, Lihua Luo, and Yang Luo

Subjects

Inflammation, biology, Somatic cell, Immunology, Receptors, Antigen, B-Cell, Somatic hypermutation, Atopic dermatitis, Immunoglobulin E, medicine.disease, Peripheral blood mononuclear cell, Dermatitis, Atopic, Psoriasis, Leukocytes, Mononuclear, medicine, biology.protein, Humans, Immunology and Allergy, Immunoglobulin heavy chain, IGHD

Abstract

Background Epicutaneous sensitization is an important route for the production of IgE, and skin inflammation-induced IgE has recently been reported having features of natural antibody. Atopic dermatitis (AD) and psoriasis have differentially increased level of serum IgE; however, the production mechanism of IgE in these inflammatory skin diseases remains unknown. Objective To explore the origin of IgE in AD and psoriasis by analyzing the B cell receptor repertoire. Methods mRNA was prepared from peripheral blood mononuclear cells of AD and psoriasis patients that had elevated serum levels of IgE, and immunoglobulin heavy chain (IGH) repertoires were sequenced after reverse transcription. Clonal lineages of B cells containing members expressing IgE were identified, and somatic hypermutations in IGH inherited from common ancestors within the clonal lineage were used to infer the relationships between B cells. Results The proportions of IGHE from AD and psoriasis were higher than that of normal control, which were positively correlated with the levels of serum total IgE. The somatic hypermutation value of IGHE variable region was lower than that of IGHG and IGHA, but higher than IGHM and IGHD, indicating a mixed natural and adaptive origins of IgE; and psoriasis demonstrated lower level of hypermutation than AD. The Shannon indexes of CDR3 in IGHE of AD and psoriasis were higher than that of normal control, also supporting the natural origin. The VH usage of IgE was weakly biased in AD and psoriasis patients with high level of house dust mite-specific IgE. Comparison of the number of shared mutations in multi-isotype lineages containing IgE showed that isotype-switching from IgG-expressing B cells might be the major source of IgE in AD and psoriasis. Conclusion IgE has heterogeneous origin in AD and psoriasis, and skin inflammation may contribute to the increased production of natural IgE.

Published

2021

40. DNA crosslinking and recombination‐activating genes 1/2 (RAG1/2) are required for oncogenic splicing in acute lymphoblastic leukemia

Author

Zhihui Li, Guoyu Meng, Zhu Chen, Yang Liang, Wei-Na Zhang, Xue Dong, Weiguo Hu, Su-Jiang Zhang, Chengli Fang, Jiang Zhu, Yu Zhang, Nuo Cheng, Jian-Qing Mi, Ling Bai, Minghao Jiang, Yajie Zhao, Jinyan Huang, Xiang-Qin Weng, Sai-Juan Chen, Hao Zhang, and Yuwen Li

Subjects

Cancer Research, DUX4/IGH, ERGalt, Carcinogenesis, Proximity ligation assay, Acute lymphoblastic leukemia, Recombination-activating gene, alternative splicing, DUX4, X-Ray Diffraction, hemic and lymphatic diseases, Scattering, Small Angle, Animals, Humans, Lectins, C-Type, RAG1/2, Gene, RC254-282, Homeodomain Proteins, Recombination, Genetic, Chemistry, Alternative splicing, Intron, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, hemic and immune systems, Original Articles, DNA, Precursor Cell Lymphoblastic Leukemia-Lymphoma, Molecular biology, Oncology, Receptors, Mitogen, RNA splicing, Immunoglobulin heavy chain, Original Article

Abstract

Background Abnormal alternative splicing is frequently associated with carcinogenesis. In B-cell acute lymphoblastic leukemia (B-ALL), double homeobox 4 fused with immunoglobulin heavy chain (DUX4/IGH) can lead to the aberrant production of E-26 transformation-specific family related gene abnormal transcript (ERGalt ) and other splicing variants. However, the molecular mechanism underpinning this process remains elusive. Here, we aimed to know how DUX4/IGH triggers abnormal splicing in leukemia. Methods The differential intron retention analysis was conducted to identify novel DUX4/IGH-driven splicing in B-ALL patients. X-ray crystallography, small angle X-ray scattering (SAXS), and analytical ultracentrifugation were used to investigate how DUX4/IGH recognize double DUX4 responsive element (DRE)-DRE sites. The ERGalt biogenesis and B-cell differentiation assays were performed to characterize the DUX4/IGH crosslinking activity. To check whether recombination-activating gene 1/2 (RAG1/2) was required for DUX4/IGH-driven splicing, the proximity ligation assay, co-immunoprecipitation, mammalian two hybrid characterizations, in vitro RAG1/2 cleavage, and shRNA knock-down assays were performed. Results We reported previously unrecognized intron retention events in C-type lectin domain family 12, member A abnormal transcript (CLEC12Aalt ) and chromosome 6 open reading frame 89 abnormal transcript (C6orf89alt ), where also harbored repetitive DRE-DRE sites. Supportively, X-ray crystallography and SAXS characterization revealed that DUX4 homeobox domain (HD)1-HD2 might dimerize into a dumbbell-shape trans configuration to crosslink two adjacent DRE sites. Impaired DUX4/IGH-mediated crosslinking abolishes ERGalt , CLEC12Aalt , and C6orf89alt biogenesis, resulting in marked alleviation of its inhibitory effect on B-cell differentiation. Furthermore, we also observed a rare RAG1/2-mediated recombination signal sequence-like DNA edition in DUX4/IGH target genes. Supportively, shRNA knock-down of RAG1/2 in leukemic Reh cells consistently impaired the biogenesis of ERGalt , CLEC12Aalt , and C6orf89alt . Conclusions All these results suggest that DUX4/IGH-driven DNA crosslinking is required for RAG1/2 recruitment onto the double tandem DRE-DRE sites, catalyzing V(D)J-like recombination and oncogenic splicing in acute lymphoblastic leukemia.

Published

2021

41. Practical Considerations for Using RNA Sequencing in Management of B-Lymphoblastic Leukemia

Author

Winnie Hui Ni Chin, Evelyn Huizi Lim, Joshua Yew Suang Lim, Bernice Ling Zhi Oh, Nan Jiang, Zhenhua Li, Kean Hui Chiew, Hany Ariffin, Allen Eng Juh Yeoh, Jun J. Yang, Shirley Kow Yin Kham, Yi Lu, and Ah Moy Tan

Subjects

Oncology, Sanger sequencing, medicine.medical_specialty, Thiopurine methyltransferase, biology, business.industry, Genetic heterogeneity, Disease, medicine.disease, Pathology and Forensic Medicine, symbols.namesake, Leukemia, Workflow, Internal medicine, medicine, symbols, biology.protein, Molecular Medicine, Immunoglobulin heavy chain, Oncogene Fusion, business

Abstract

Despite the immense genetic heterogeneity of B-lymphoblastic leukemia [or precursor B-cell acute lymphoblastic leukemia (B-ALL)], RNA sequencing (RNA-Seq) could comprehensively interrogate its genetic drivers, assigning a specific molecular subtype in >90% of patients. However, study groups have only started to use RNA-Seq. For broader clinical use, technical, quality control, and appropriate performance validation are needed. We describe the development and validation of an RNA-Seq workflow for subtype classification, TPMT/NUDT15/TP53 variant discovery, and immunoglobulin heavy chain (IGH) disease clone identification for Malaysia-Singapore acute lymphoblastic leukemia (ALL) 2020. We validated this workflow in 377 patients in our preceding Malaysia-Singapore ALL 2003/Malaysia-Singapore ALL 2010 studies and proposed the quality control measures for RNA quality, library size, sequencing, and data analysis using the International Organization for Standardization 15189 quality and competence standard for medical laboratories. Compared with conventional methods, we achieved >95% accuracy in oncogene fusion identification, digital karyotyping, and TPMT and NUDT15 variant discovery. We found seven pathogenic TP53 mutations, confirmed with Sanger sequencing, which conferred a poorer outcome. Applying this workflow prospectively to the first 21 patients in Malaysia-Singapore ALL 2020, we identified the genetic drivers and IGH disease clones in >90% of patients with concordant TPMT, NUDT15, and TP53 variants using PCR-based methods. The median turnaround time was 12 days, which was clinically actionable. In conclusion, RNA-Seq workflow could be used clinically in management of B-cell ALL patients.

Published

2021

42. Dual Primary IGH Translocations in Multiple Myeloma: A Novel Finding

Author

Aishwarya Ravindran, Shaji Kumar, Nicholas Wongchaowart, James B. Smadbeck, Jess F. Peterson, Patricia T. Greipp, Linda B. Baughn, and Rhett P. Ketterling

Subjects

Cancer Research, medicine.medical_specialty, business.industry, Cytogenetics, Chromosomal translocation, Hematology, Middle Aged, Plasma cell neoplasm, medicine.disease, Mutually exclusive events, Translocation, Genetic, Clinical Practice, Oncology, immune system diseases, hemic and lymphatic diseases, Cancer research, medicine, Humans, Immunoglobulin heavy chain, Female, Immunoglobulin Heavy Chains, Multiple Myeloma, business, Multiple myeloma

Abstract

Clinical Practice Points • Cytogenetics in multiple myeloma is utilized to risk stratify patients into standard and high-risk groups. • Immunoglobulin heavy chain (IGH) gene translocations such as t(4;14) and t(14;16) are high-risk cytogenetic abnormalities that confer poor outcomes to therapy in multiple myeloma. • Primary IGH translocations are typically considered mutually exclusive events. • Here, we describe a case of multiple myeloma with dual primary IGH translocations involving both t(4;14) and t(14;16).

Published

2021

43. Prevalent, protective, and convergent IgG recognition of SARS-CoV-2 non-RBD spike epitopes

Author

Lori A. Rowe, Ilya J. Finkelstein, Kamyab Javanmardi, Daniel R. Boutz, Jin Eyun Kim, Shivaprakash Gangappa, Jonathan R. McDaniel, Ralph S. Baric, Dhwani Batra, Maria D. Person, George Georgiou, William N. Voss, Brent L. Iverson, Gregory C. Ippolito, Katia George, Andrew S. Herbert, Yuri Tanno, Foteini Bartzoka, Shawn A. Abbasi, Jason S. McLellan, Jimmy Gollihar, Suryaprakash Sambhara, Daniel Billick, Jule Goike, Chelsea J. Paresi, Whitney Pickens, George Delidakis, Justin S. Lee, Nicole V. Johnson, Yixuan J. Hou, Nianshuang Wang, Andrew P. Horton, Jason J. Lavinder, Jan Pohl, Michelle Gadush, Chia Wei Chou, John M. Dye, and Dalton M Towers

Subjects

Proteomics, Protein domain, Antibody Affinity, Immunoglobulin Variable Region, Antibodies, Viral, medicine.disease_cause, Article, Epitope, Immunoglobulin G, Epitopes, Mice, Protein Domains, medicine, Animals, Humans, Immune Evasion, chemistry.chemical_classification, Mice, Inbred BALB C, Mutation, Multidisciplinary, biology, SARS-CoV-2, Repertoire, Antibodies, Monoclonal, COVID-19, Antibodies, Neutralizing, Virology, chemistry, Spike Glycoprotein, Coronavirus, biology.protein, Immunoglobulin heavy chain, Antibody, Immunoglobulin Heavy Chains, Glycoprotein

Abstract

Although humoral immunity is essential for control of SARS-CoV-2, the molecular composition, binding epitopes and effector functions of the immunoglobulin G (IgG) antibodies that circulate in blood plasma following infection are unknown. Proteomic deconvolution of the circulating IgG repertoire (Ig-Seq (1) ) to the spike ectodomain (S-ECD (2) ) in four convalescent study subjects revealed that the plasma response is oligoclonal and directed predominantly (>80%) to S-ECD epitopes that lie outside the receptor binding domain (RBD). When comparing antibodies directed to either the RBD, the N-terminal domain (NTD) or the S2 subunit (S2) in one subject, just four IgG lineages (1 anti-S2, 2 anti-NTD and 1 anti-RBD) accounted for 93.5% of the repertoire. Although the anti-RBD and one of the anti-NTD antibodies were equally potently neutralizing in vitro , we nonetheless found that the anti-NTD antibody was sufficient for protection to lethal viral challenge, either alone or in combination as a cocktail where it dominated the effect of the other plasma antibodies. We identified in vivo protective plasma anti-NTD antibodies in 3/4 subjects analyzed and discovered a shared class of antibodies targeting the NTD that utilize unmutated or near-germline IGHV1-24, the most electronegative IGHV gene in the human genome. Structural analysis revealed that binding to NTD is dominated by interactions with the heavy chain, accounting for 89% of the entire interfacial area, with germline residues uniquely encoded by IGHV1-24 contributing 20% (149 Å (2) ). Together with recent reports of germline IGHV1-24 antibodies isolated by B-cell cloning (3,4) our data reveal a class of shared IgG antibodies that are readily observed in convalescent plasma and underscore the role of NTD-directed antibodies in protection against SARS-CoV-2 infection.

Published

2021

44. Linked-read whole-genome sequencing resolves common and private structural variants in multiple myeloma

Author

Peña-Pérez, L., Frengen, N., Hauenstein, J., Gran, C., Gustafsson, C., Eisfeldt, J., Kierczak, M., Taborsak-Lines, F., Olsen, Remi-André, Wallblom, A., Krstic, A., Ewels, Philip, Lindstrand, A., Månsson, R., Peña-Pérez, L., Frengen, N., Hauenstein, J., Gran, C., Gustafsson, C., Eisfeldt, J., Kierczak, M., Taborsak-Lines, F., Olsen, Remi-André, Wallblom, A., Krstic, A., Ewels, Philip, Lindstrand, A., and Månsson, R.

Abstract

Multiple myeloma (MM) is an incurable and aggressive plasma cell malignancy characterized by a complex karyotype with multiple structural variants (SVs) and copy-number variations (CNVs). Linked-read whole-genome sequencing (lrWGS) allows for refined detection and reconstruction of SVs by providing long-range genetic information from standard short-read sequencing. This makes lrWGS an attractive solution for capturing the full genomic complexity of MM. Here we show that high-quality lrWGS data can be generated from low numbers of cells subjected to fluorescence-activated cell sorting (FACS) without DNA purification. Using this protocol, we analyzed MM cells after FACS from 37 patients with MM using lrWGS. We found high concordance between lrWGS and fluorescence in situ hybridization (FISH) for the detection of recurrent translocations and CNVs. Outside of the regions investigated by FISH, we identified .150 additional SVs and CNVs across the cohort. Analysis of the lrWGS data allowed for resolution of the structure of diverse SVs affecting the MYC and t(11;14) loci, causing the duplication of genes and gene regulatory elements. In addition, we identified private SVs causing the dysregulation of genes recurrently involved in translocations with the IGH locus and show that these can alter the molecular classification of MM. Overall, we conclude that lrWGS allows for the detection of aberrations critical for MM prognostics and provides a feasible route for providing comprehensive genetics. Implementing lrWGS could provide more accurate clinical prognostics, facilitate genomic medicine initiatives, and greatly improve the stratification of patients included in clinical trials.

Published

2022

45. Coupled analysis of transcriptome and BCR mutations reveals role of OXPHOS in affinity maturation

Author

Dianyu Chen, Di Xu, Godhev K. Manakkat Vijay, Fu Shujie, Heping Xu, Yan Wang, Colt W. Nash, Danyang He, Nathan Salomonis, and Harinder Singh

Subjects

0301 basic medicine, Cell division, Immunology, Somatic hypermutation, Germinal center, Cell cycle, Biology, Cell biology, Transcriptome, Affinity maturation, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, medicine.anatomical_structure, medicine, Immunology and Allergy, Immunoglobulin heavy chain, B cell, 030215 immunology

Abstract

Antigen-activated B cells diversify variable regions of B cell antigen receptors by somatic hypermutation in germinal centers (GCs). The positive selection of GC B cells that acquire high-affinity mutations enables antibody affinity maturation. In spite of considerable progress, the genomic states underlying this process remain to be elucidated. Single-cell RNA sequencing and topic modeling revealed increased expression of the oxidative phosphorylation (OXPHOS) module in GC B cells undergoing mitoses. Coupled analysis of somatic hypermutation in immunoglobulin heavy chain (Igh) variable gene regions showed that GC B cells acquiring higher-affinity mutations had further elevated expression of OXPHOS genes. Deletion of mitochondrial Cox10 in GC B cells resulted in reduced cell division and impaired positive selection. Correspondingly, augmentation of OXPHOS activity with oltipraz promoted affinity maturation. We propose that elevated OXPHOS activity promotes B cell clonal expansion and also positive selection by tuning cell division times. Xu and colleagues use single-cell transcriptomic analyses to uncover distinct expression dynamics of metabolic programs in germinal center B cells. Coupled analysis of transcriptional states and Igh variable sequences revealed that OXPHOS metabolism is enhanced in GC B cells undergoing positive selection. Their findings suggest BCR signaling tunes GC B cell metabolism to accelerate the cell cycle of positively selected GC B cells.

Published

2021

46. Evolutionary clonal trajectories in nodular lymphocyte-predominant Hodgkin lymphoma with high risk of transformation

Author

Dennis A. Eichenauer, Donjete Simnica, Sylvia Hartmann, Alfred C. Feller, Claudia Wickenhauser, Wolfram Klapper, Martine Vornanen, Andreas Rosenwald, Edith Willscher, Julia Bein, Mascha Binder, Benjamin Thiele, Lisa Paschold, German Ott, Heinz Wolfram Bernd, Falko Fend, Tampere University, Department of Pathology, and Clinical Medicine

Subjects

medicine.medical_specialty, Cell of origin, Immunoglobulin D, Somatic evolution in cancer, Article, Diagnosis, Differential, 03 medical and health sciences, 0302 clinical medicine, Internal medicine, medicine, Humans, Lymphocytes, Biology, Phylogeny, Genetics, Hematology, biology, Editorials, medicine.disease, Hodgkin Disease, Lymphoma, Transformation (genetics), biology.protein, Immunoglobulin heavy chain, 3111 Biomedicine, Lymph Nodes, Neoplasm Recurrence, Local, Clone (B-cell biology), 030215 immunology

Abstract

The B-cell architecture of nodular lymphocyte-predominant Hodgkin lymphoma (NLPHL) is complex since it is composed of malignant lymphocyte-predominant cells along with a rich B-cell bystander environment. To gain insight into molecular determinants of disease transformation, we studied B-cell evolutionary trajectories in lymphoma tissue from diagnosis to relapse or transformation to non-Hodgkin lymphoma by next-generation sequencing of immunoglobulin heavy chains. Patients with NLPHL that later transformed were older and showed IgD negativity, absence of the characteristic IGHV3/IGHD3/IGHJ6 lymphocyte-predominant rearrangement and high repertoire clonality. We constructed phylogenetic trees within the compartment of the malignant clone to investigate clonal evolution. In all relapsing cases, the lymphocyte-predominant rearrangement was identical at diagnosis and relapse. NLPHL cases with transformation showed more complex trajectories with strong intraclonal diversification. The dominant founder clone in transformations showed clonal evolution if derived from the same cell of origin, or arose from a different cell of origin. Together, our data point to a significant role of antigenic drive in the transformation of NLHPL and identify high B-cell repertoire clonality with dominant intraclonal lymphocyte-predominant cell diversification as a hallmark of transformation. Sequencing of initial paraffin-embedded tissue may therefore be applied diagnostically to identify NLPHL cases with high risk of transformation. publishedVersion

Published

2021

47. First-time application of a PCR-based clonality assay in a large cohort of non-domestic felines

Author

Barbara C. Rütgen, Anna Kübber-Heiss, Annika Posautz, Sophia Unterkreuter, Sandra Groiss, and Sabine E. Hammer

Subjects

Male, Felidae, medicine.medical_specialty, Lymphoma, 040301 veterinary sciences, Biology, Polymerase Chain Reaction, Sensitivity and Specificity, Cohort Studies, 0403 veterinary science, 03 medical and health sciences, medicine, Animals, Lymphocytes, 030304 developmental biology, Gene Rearrangement, 0303 health sciences, CATS, General Veterinary, Feline Lymphoma, Receptors, Antigen, T-Cell, gamma-delta, 04 agricultural and veterinary sciences, Gold standard (test), medicine.disease, Virology, T-Cell Receptor Gamma Chain, Immunoglobulin heavy chain, Female, Histopathology, Primer (molecular biology)

Abstract

Feline lymphoma, one of the most important malignant tumors in domestic cats, is also increasingly diagnosed in non-domestic felines, most notably, African lions (Panthera leo). The gold standard for the diagnosis of lymphoma is histopathological evaluation. As an additional tool, the PCR for antigen receptor gene rearrangement (PARR) has been established. To support the diagnosis on a molecular level, the PCR-based clonality assay is designed to distinguish between reactive and neoplastic lymphocyte populations. In general, PARR primers are used to target complete immunoglobulin heavy chain V-D-J (IGH-VDJ) and T-cell receptor gamma V-J (TRG-VJ) chain gene rearrangements. In this study, we validated the primer sets used in routine diagnostics of domestic cats for the application in non-domestic felines. Clonality testing was used in 41 non-domestic feline species and the results were interpreted in the light of their clinical history and their pathology. In total, clonality could be detected in 8 non-domestic felines (19.4%), including 3 lymphoma cases confirmed by histopathology. These results confirmed the successful application of domestic feline-specific PARR primers in non-domestic feline species. Diagnostic sensitivity and specificity of the clonality assay were 100% and 88%, respectively. Finally, the overall diagnostic accuracy was 89%.

Published

2021

48. Quantification of Residual Tumor Cells in Monoclonal B-cell Lymphoma

Author

Pfitzner, Thomas, Engert, Andreas, Barth, Stefan, Meuer, Stefan, editor, Wittwer, Carl, editor, and Nakagawara, Kan-Ichi, editor

Published

2001

49. Development and evaluation of polyclonal antisera for detection of the IgM heavy chain of multiple fish species.

Author

Jirapongpairoj, Walissara, Hirono, Ikuo, and Kondo, Hidehiro

Subjects

*IMMUNE response in fishes, *IMMUNE serums, *IMMUNOGLOBULIN M, *WESTERN immunoblotting, *ENZYME-linked immunosorbent assay

Abstract

Antibodies are widely considered to be essential tools for detection of immune responses in various fish species. Here we produced the peptide polyclonal antisera (anti-fish IgH-1 and anti-fish IgH-2) to detect IgM of various fish species. The peptides were designed based on the conserved sequence of the fish immunoglobulin heavy chains of seven fish species (Japanese flounder, seabream, yellowtail, carp, rainbow trout, hybrid sturgeon and banded houndshark). By Western blotting, anti-fish IgH-1 antiserum detected the IgMs of all fish species except banded houndshark. Anti-fish IgH-2 antiserum clearly reacted with the IgMs of only three of the fish species (seabream, yellowtail and rainbow trout). Attempts to use the antisera to measure fish antibody titer by ELISA were unsuccessful. These results demonstrate that anti-fish IgH-1 peptide polyclonal antiserum is a potentially applicable tool for detecting immunoglobulins in various fish species by Western blotting. [ABSTRACT FROM AUTHOR]

Published

2017

50. Competitive Promoter-Associated Matrix Attachment Region Binding of the Arid3a and Cux1 Transcription Factors.

Author

Dongkyoon Kim, Schmidt, Christian, Brown, Mark A., and Tucker, Haley

Subjects

IMMUNOGLOBULIN heavy chains, MATRIX attachment regions, B cells, LIPOPOLYSACCHARIDES, GENE expression, PHYSIOLOGY

Abstract

Arid3a/Bright/Dril1 is a B cell-specific transactivator that regulates immunoglobulin heavy chain (IgH) gene transcription by binding promoter and enhancer-associated matrix attachment regions (MARs) within the IgH gene locus. Promoter MAR-mediated Arid3a transactivation is antagonized by direct competition of MAR binding by Cux1/CDP--a ubiquitously expressed repressor originally termed NF-μNR. We report that the NF-μNR complex includes Arid3a in B cells but not in non-B cells through mobility shift assays. The binding activity of NF-μNR and Arid3a in B cells is reciprocally altered during the cell division cycle and by the B cell mitogen lipopolysaccharide LPS. LPS treatment had no effect on Arid3a localization but increased its total abundance within the nucleus and cytoplasm. We show that this increased level of Arid3a is capable of displacing Cux from the MARs to facilitate IgH gene transcription. Finally, we showed that the MARs (termed Bf150 and Tx125) associated with the VH1 rearranged variable region expressed in the S107 murine plasmacytoma, can repress reporter gene transcription in non-B cells and that they can relieve the repression mediated by Eμ enhancer in B cells. These results have significant implications for early human development and demonstrate that MARs in IgH locus, NF-μNR and Arid3a regulate IgH gene expression in a concerted fashion. This paves the way for future studies examining the misregulation of this pathway in pediatric disease. [ABSTRACT FROM AUTHOR]

Published

2017