HLA antigen expression at the single cell level on a K562 × B cell hybrid: An analysis with monoclonal antibodies using bacterial binding assays

1982 ◽  
Vol 8 (6) ◽  
pp. 775-789 ◽  
Author(s):  
Andreas Ziegler ◽  
Barbara Uchańska-Ziegler ◽  
Jesper Zeuthen ◽  
Peter Wernet
Keyword(s):  
Monoclonal Antibodies ◽  
B Cell ◽  
Single Cell ◽  
Cell Hybrid ◽  
Antigen Expression ◽  
Single Cell Level ◽  
Binding Assays ◽  
Cell Level ◽  
Hla Antigen ◽  
Bacterial Binding

scholarly journals Cellular Barcoding Links B-1a B Cell Potential to a Fetal Hematopoietic Stem Cell State at the Single-Cell Level

Immunity ◽  
2016 ◽  
Vol 45 (2) ◽  
pp. 346-357 ◽  
Author(s):  
Trine A. Kristiansen ◽  
Elin Jaensson Gyllenbäck ◽  
Alya Zriwil ◽  
Tomas Björklund ◽  
Jeremy A. Daniel ◽  
...  
Keyword(s):  
Stem Cell ◽  
B Cell ◽  
Single Cell ◽  
Hematopoietic Stem Cell ◽  
Single Cell Level ◽  
Cell Level ◽  
Cell Potential ◽  
Hematopoietic Stem ◽  
Stem Cell State ◽  
Cellular Barcoding

Selective inhibition of natural killer activity by the monoclonal antibodies OKT10 and VEP10 at the single cell level

1984 ◽  
Vol 88 (2) ◽  
pp. 382-392 ◽  
Author(s):  
Marc G. Golightly ◽  
Hlllel S. Koren ◽  
William W. Travis ◽  
C.Philip Brandt ◽  
Barton F. Haynes ◽  
...  
Keyword(s):  
Monoclonal Antibodies ◽  
Single Cell ◽  
Natural Killer ◽  
Natural Killer Activity ◽  
Selective Inhibition ◽  
Single Cell Level ◽  
Cell Level ◽  
Killer Activity

A microfluidic chip for screening high-producing hybridomas at single cell level

Lab on a Chip ◽  
2020 ◽  
Vol 20 (21) ◽  
pp. 4043-4051
Author(s):  
Weikai Zhang ◽  
Ren Li ◽  
Fei Jia ◽  
Zhiyuan Hu ◽  
Qin Li ◽  
...  
Keyword(s):  
Monoclonal Antibodies ◽  
Targeted Therapy ◽  
Single Cell ◽  
Laboratory Study ◽  
Microfluidic Chip ◽  
Single Cell Level ◽  
Cell Level ◽  
Biomedical Study

Hybridomas are a commonly used, or even the only option, for laboratory study and pilot production of monoclonal antibodies (mAbs), which are crucial for both targeted therapy and biomedical study.

scholarly journals "Snapshotting" Somatic Hypermutation in Single Follicular Lymphoma Cells

Blood ◽  
2021 ◽  
Vol 138 (Supplement 1) ◽  
pp. 1151-1151
Author(s):  
Juleta H. Sepulveda-Yanez ◽  
Diego Alvarez-Saravia ◽  
Edwin Quinten ◽  
Roberta Menafra ◽  
Susan L. Kloet ◽  
...  
Keyword(s):  
Follicular Lymphoma ◽  
B Cell ◽  
Single Cell ◽  
Germinal Center ◽  
Somatic Mutations ◽  
Somatic Hypermutation ◽  
Single Cell Level ◽  
Cell Level ◽  
Single Nucleotide

Abstract Introduction Follicular Lymphoma (FL) is one of the most prevalent B-cell neoplasms and despite recent advances remains incurable in most cases. FL cells are malignant counterparts of normal germinal center B-cells. At molecular level FL are characterized by the t(14;18) which results in the overexpression of the BCL-2. These apoptosis resistant cells accumulate somatic mutations associated with tumorigenesis and progression. Whereas several mutagenic mechanisms shape the FL genomic landscape, up to 22% of the mutations may be attributed to activation-induced cytidine deaminase (AID) activity. Under physiological conditions AID is responsible for somatic hypermutation (SHM) in immunoglobulin genes (IG) of germinal center B-cells. In fact, it is accepted that ongoing SHM still occurs at relatively high rates in FL cells as compared with other germinal center lymphoid neoplasms. Moreover, we recently demonstrated the direct effect of AID overexpression inducing somatic mutations driving murine and human B-cell neoplasm progression in vivo. Therefore, unveiling the molecular basis of AID activity in lymphoma cells remains essential to understand lymphomagenesis and to develop novel targeted therapies. The advent of single-cell high-throughput sequencing has enabled the analysis of molecular events at an unprecedented resolution. Therefore, we designed a study to capture AID-induced somatic hypermutation at the single cell level in FL. Methods Tumor samples derived from 14 FL patients were analyzed, as controls, we chose a B-cell malignancy with lower SHM rates and included 5 samples derived from chronic lymphocytic leukemia (CLL) and 2 from monoclonal B lymphocytosis (MBL). Single cell whole cDNA libraries were obtained by 10X Genomics. Immunoglobulin gene single cell libraries were prepared by enrichment with seminested amplification using 3 ′ constant domain primers followed by 10X Genomics prep. Both single-cell libraries were sequenced in paired-end mode (2 × 150 bp) on an Illumina Hiseq platform. We developed an immunoglobulin alignment tool to enable the analysis of highly mutated IG sequences derived from FL. A consensus sequence was obtained by transcript associated with a unique molecular identifier (UMI) for every cell. Then, the presence of variants in the IG by position in a particular cell was annotated. These observations were filtered using quality parameters (read depth => 25 , frequency of the event => 20%, UMIs supporting every variant => 5). Results We analyzed an average of 926 cells per case. Our data confirms at the single cell level previous reports on high clonal heterogeneity and hypermutation rate (mean 18.7%) in FL. When analyzing intracellular heterogeneity we observed single FL cells expressing simultaneously transcripts derived from the same immunoglobulin VDJ rearrangement but displaying high confidence single nucleotide variants. After applying strict filtering strategies to account for potential technical issues we defined the occurrence of "SHM snapshot events'' when a single cell displayed a set of transcripts from a particular VDJ rearrangement with and without the occurring single nucleotide variant. Such events were detected in 8 of the 14 FL analyzed samples. In those 8 samples, 114 events were observed in which two different transcripts of one specific IG were found within a single cell. AID-related motifs (WRCY, WA and RCG) were found in 45% of the SHM snapshot events. SHM snapshot events were undetectable in CLL (5 samples) and 3 SHM snapshot events were detected in MBL (2 samples). In addition, the occurrence of SHM snapshot events was significantly associated with AID expression (Fisher exact test, p-value < 0.001). On the other hand, AID expression was not detectable on CLL and MBL samples. Conclusion Here we report for the first time the occurrence of ongoing somatic hypermutation at a single cell level in FL. The simultaneous detection of both the pre and post mutation IG mRNA transcripts within a single cell may be indicative of SHM occurring more recently than the lifespan of mRNA transcript. The detection of this phenomenon in 57% of FL samples and its association with AID expression suggests that AID-induced mutagenesis may be acting at a much higher rate than expected. This work highlights the role of AID in shaping the tumor heterogeneity in FL and the need to further understand the role of this enzyme in lymphomagenesis and tumor progression. Disclosures No relevant conflicts of interest to declare.

scholarly journals Single-Cell Decoding of Minimal Residual Disease in Pediatric B Cell Acute Lymphoblastic Leukemia

Blood ◽  
2021 ◽  
Vol 138 (Supplement 1) ◽  
pp. 2385-2385
Author(s):  
Yingchi Zhang ◽  
Shicheng Wang ◽  
Jingliao Zhang ◽  
Chao Liu ◽  
Xinqi Li ◽  
...  
Keyword(s):  
B Cells ◽  
B Cell ◽  
Single Cell ◽  
Pediatric Cancer ◽  
Residual Disease ◽  
Lymphoblastic Leukemia ◽  
Leukemic Cells ◽  
Single Cell Level ◽  
Cell Level ◽  
Differentiation Stage

Abstract Acute lymphoblastic leukemia (ALL) is the most common pediatric cancer, of which B cell ALL (B-ALL) accounts for up to 85% of all cases. Although risk-stratified chemotherapy significantly improves the clinical outcome of affected pediatric patients with B-ALL, relapse still occurs in approximately 10% of children, representing the main cause of pediatric cancer deaths. Minimal residual disease (MRD) that persists after chemotherapy was the most valuable prognostic marker for hematological malignancies and solid cancers. Unfortunately, our understanding of the resistance mechanisms elicited in MRD is limited due to the rarity and heterogeneity of these residual cells. In our study, we employed paired scRNA-seq and single-cell BCR sequencing (scBCR-seq) to study the distinct features of leukemic cells from longitudinal samples obtained at the diagnosis, residual and relapsed stages at the single-cell level. By performing unsupervised clustering of the scRNA-seq data from 16,543 bone marrow CD19 -CD34 +cells and 20,392 CD19 +cells of healthy donors, we successfully defined the cell clusters of different B cell development stages sequentially, from hematopoietic stem cell / lymphoid-primed multipotential progenitors (HSC/LMPP) to common lymphoid progenitor (CLP), proB, preBI, preBII, immature/mature B cells and finally, activated B cells. By referring to the landmarks of normal cells, we then employed scRNA-seq and scBCR-seq to further dissect the phenotypic complexities within and across 4 pediatric B-ALL diagnostic-relapsed pairs at the single cell level. Our study found that BCR states can be used to distinguish leukemic cells and normal cells. From the four relapsed pediatric B-ALL patients, we obtained a total of 104,055 CD19 +cells with paired scRNA-seq and scBCR-seq data encompassing the three stages of B cell differentiation that passed the quality control. By examining the scBCR-seq data at the diagnosis stage to distinguish leukemic and normal (or non-leukemic) B cells based on genome-wide expression patterns rather than a few marker genes, we employed a machine learning approach. To train the classifier, CD19 +cells with non-clonal BCRs in D19 samples were selected as "non-leukemic", and CD19 +cells with clonal BCRs (B265) and without detected BCRs (B590, B069 and B887) in D19 samples were selected as "leukemic". Using this strategy, we compared the gene expression profiles of the leukemic cells at the diagnosis and relapse for each patient, with the aim to identify specific features of relapse stage leukemia cells at the single-cell level. We found that the cell composition profile tended to shift to early differentiation stages in the relapsed samples in all four patients. By analyzing the differentiation stage, cell cycle and gene expression characteristics of relapsed cell samples at the single-cell level, we obtained some unique findings, such as significantly increased expression of CDKN1A in relapsed cells. To understand the basis of such specific differentiation stage and cell cycle transition during chemotherapy, we performed differential expression analysis to identify genes specifically altered at D19 compared to diagnosis and relapse. Then, pathway enrichment analysis applied to the differentially expressed genes revealed that the hypoxia pathway was one of the top hits, being significantly upregulated during intensified chemotherapy. We obtained experimental support by validating the efficacy of the HIF-1a inhibitor PX478 combined with chemotherapy drugs in two B-ALL cell lines and two primary B-ALL cells. In summary, our study leveraged single-cell transcriptomic analysis with paired BCR repertoire profiling to decode the molecular aberrations across the phenotypically heterogeneous disease, B-ALL. We also applied a powerful B cell development classifier and an innovative machine learning model for B-ALL cell identification at single-cell resolution to determine the clonal signatures, and to track residual cell evolution in a longitudinal manner from diagnosis, to post-treatment, and finally relapse. We propose that hypoxia signaling pathway activation might serve as valuable MRD therapeutic target. While this study provided great insights into the transcriptomic characteristics of MRD cells, practically, our analytical approach could readily be applied to other hematological malignancies and solid cancers. Disclosures No relevant conflicts of interest to declare.

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