Your search keyword '"Limiting dilution"' showing total 399 results

1. A Method to Generate and Rescue Recombinant Adenovirus Devoid of Replication-Competent Particles in Animal-Origin-Free Culture Medium.

Author

Elahi, Seyyed Mehdy, Jiang, Jennifer, Nazemi-Moghaddam, Nazila, and Gilbert, Rénald

Subjects

*SERUM-free culture media, *ADENOVIRUSES, *CELL suspensions, *CELL lines, *GENE therapy, *DNA vaccines

Abstract

Adenoviruses are promising vectors for vaccine production and gene therapy. Despite all the efforts in removing animal-derived components such as fetal bovine serum (FBS) during the production of adenovirus vector (AdV), FBS is still frequently employed in the early stages of production. Conventionally, first-generation AdVs (E1 deleted) are generated in different variants of adherent HEK293 cells, and plaque purification (if needed) is performed in adherent cell lines in the presence of FBS. In this study, we generated an AdV stock in SF-BMAdR (A549 cells adapted to suspension culture in serum-free medium). We also developed a limiting dilution method using the same cell line to replace the plaque purification assay. By combining these two technologies, we were able to completely remove the need for FBS from the process of generating and producing AdVs. In addition, we demonstrated that the purified AdV stock is free of any replication-competent adenovirus (RCA). Furthermore, we demonstrated that our limiting dilution method could effectively rescue an AdV from a stock that is highly contaminated with RCA. [ABSTRACT FROM AUTHOR]

Published

2023

2. Transcriptomics at the Single Cell Level and Human Diseases: Opportunities and Challenges in Data Processing and Analysis

Author

Maracaja-Coutinho, Vinicius, Severino, Patricia, and Passos, Geraldo A., editor

Published

2022

3. The Parasite Reduction Ratio (PRR) Assay Version 2: Standardized Assessment of Plasmodium falciparum Viability after Antimalarial Treatment In Vitro.

Author

Walz, Annabelle, Duffey, Maëlle, Aljayyoussi, Ghaith, Sax, Sibylle, Leroy, Didier, Besson, Dominique, Burrows, Jeremy N., Cherkaoui-Rbati, Mohammed H., Gobeau, Nathalie, Westwood, Marie-Anne, Siethoff, Christoph, Gamo, Francisco-Javier, Mäser, Pascal, and Wittlin, Sergio

Subjects

*PLASMODIUM falciparum, *PARASITES, *PLASMODIUM, *QUALITY control

Abstract

With artemisinin-resistant Plasmodium falciparum parasites emerging in Africa, the need for new antimalarial chemotypes is persistently high. The ideal pharmacodynamic parameters of a candidate drug are a rapid onset of action and a fast rate of parasite killing or clearance. To determine these parameters, it is essential to discriminate viable from nonviable parasites, which is complicated by the fact that viable parasites can be metabolically inactive, whilst dying parasites can still be metabolically active and morphologically unaffected. Standard growth inhibition assays, read out via microscopy or [3H] hypoxanthine incorporation, cannot reliably discriminate between viable and nonviable parasites. Conversely, the in vitro parasite reduction ratio (PRR) assay is able to measure viable parasites with high sensitivity. It provides valuable pharmacodynamic parameters, such as PRR, 99.9% parasite clearance time (PCT99.9%) and lag phase. Here we report the development of the PRR assay version 2 (V2), which comes with a shorter assay duration, optimized quality controls and an objective, automated analysis pipeline that systematically estimates PRR, PCT99.9% and lag time and returns meaningful secondary parameters such as the maximal killing rate of a drug (Emax) at the assayed concentration. These parameters can be fed directly into pharmacokinetic/pharmacodynamic models, hence aiding and standardizing lead selection, optimization, and dose prediction. [ABSTRACT FROM AUTHOR]

Published

2023

4. A Method to Generate and Rescue Recombinant Adenovirus Devoid of Replication-Competent Particles in Animal-Origin-Free Culture Medium

Author

Seyyed Mehdy Elahi, Jennifer Jiang, Nazila Nazemi-Moghaddam, and Rénald Gilbert

Subjects

adenovirus vector, replication-competent adenovirus, limiting dilution, animal-origin-free culture media, Microbiology, QR1-502

Abstract

Adenoviruses are promising vectors for vaccine production and gene therapy. Despite all the efforts in removing animal-derived components such as fetal bovine serum (FBS) during the production of adenovirus vector (AdV), FBS is still frequently employed in the early stages of production. Conventionally, first-generation AdVs (E1 deleted) are generated in different variants of adherent HEK293 cells, and plaque purification (if needed) is performed in adherent cell lines in the presence of FBS. In this study, we generated an AdV stock in SF-BMAdR (A549 cells adapted to suspension culture in serum-free medium). We also developed a limiting dilution method using the same cell line to replace the plaque purification assay. By combining these two technologies, we were able to completely remove the need for FBS from the process of generating and producing AdVs. In addition, we demonstrated that the purified AdV stock is free of any replication-competent adenovirus (RCA). Furthermore, we demonstrated that our limiting dilution method could effectively rescue an AdV from a stock that is highly contaminated with RCA.

Published

2023

5. Proteome alterations during clonal isolation of established human pancreatic cancer cell lines.

Author

Bernhard, P., Feilen, T., Rogg, M., Fröhlich, K., Cosenza-Contreras, M., Hause, F., Schell, C., and Schilling, O.

Abstract

Clonal isolation is an integral step of numerous workflows in genome editing and cell engineering. It comprises the isolation of a single progenitor cell from a defined cell line population with subsequent expansion to obtain a monoclonal cell population. This process is associated with transient loss of cell–cell contacts and absence of a multicellular microenvironment. Previous studies have revealed transcriptomic changes upon clonal isolation with cell line specific extent. Since transcriptome alterations are only partially reflected on the proteome level, we sought to investigate the impact of clonal isolation on the cellular proteome to a depth of > 6000 proteins in three established pancreatic cancer cell lines. We show that clonal isolation does have an impact on the cellular proteome, however, with cell line specific extent, affecting different biological processes, and also depending on the isolation method. We demonstrate a different impact of clonal isolation on mesenchymal- and epithelial-derived cell lines mainly affecting cell proliferation, metabolism, cell adhesion and cellular stress. The results bear relevance to the field of genomic editing and cell engineering and highlight the need to consider the impact of clonal isolation when interpreting data stemming from experiments that include this step. [ABSTRACT FROM AUTHOR]

Published

2022

6. A Bench-Top Approach for Isolation of Single Antibody Producing Chinese Hamster Ovary (CHO) Cells Using a Microwell-Based Microfluidic Device.

Author

Fuadiyah, Salma, Chotchindakun, Kittipat, Phatthanakun, Rungrueang, Kuntanawat, Panwong, and Yamabhai, Montarop

Subjects

MICROFLUIDIC devices, CELL suspensions, MONOCLONAL antibodies, CELL lines, CELL separation, DRUG development

Abstract

Genetically-modified monoclonal cell lines are currently used for monoclonal antibody (mAbs) production and drug development. The isolation of single transformed cells is the main hindrance in the generation of monoclonal lines. Although the conventional limiting dilution method is time-consuming, laborious, and skill-intensive, high-end approaches such as fluorescence-activated cell sorting (FACS) are less accessible to general laboratories. Here, we report a bench-top approach for isolating single Chinese hamster ovary (CHO) cells using an adapted version of a simple microwell-based microfluidic (MBM) device previously reported by our group. After loading the cell suspension to the device, the electrostatically trapped cells can be viewed under a microscope and transferred using a micropipette for further clone establishment. Compared to the conventional method, the invented approach provided a 4.7-fold increase in the number of single cells isolated per round of cell loading and demonstrated a 1.9-fold decrease in total performing time. Additionally, the percentage of correct single-cell identifications was significantly improved, especially in novice testers, suggesting a reduced skill barrier in performing the task. This novel approach could serve as a simple, affordable, efficient, and less skill-intensive alternative to the conventional single-cell isolation for monoclonal cell line establishment. [ABSTRACT FROM AUTHOR]

Published

2022

7. HepG2-NTCP Subclones Exhibiting High Susceptibility to Hepatitis B Virus Infection.

Author

Zahoor, Muhammad Atif, Kuipery, Adrian, Mosa, Alexander I., Gehring, Adam J., and Feld, Jordan J.

Subjects

*HEPATITIS B, *CELL culture, *VIRAL antigens, *HEPATITIS B virus

Abstract

HepG2 cells reconstituted with Hepatitis B virus (HBV) entry receptor sodium taurocholate co-transporting polypeptide (NTCP) are widely used as a convenient in vitro cell culture infection model for HBV replication studies. As such, it is pertinent that HBV infectivity is maintained at steady-state levels for an accurate interpretation of in vitro data. However, variations in the HBV infection efficiency due to imbalanced NTCP expression levels in the HepG2 cell line may affect experimental results. In this study, we performed single cell-cloning of HepG2-NTCP-A3 parental cells via limiting dilution and obtained multiple subclones with increased permissiveness to HBV. Specifically, one subclone (HepG2-NTCP-A3/C2) yielded more than four-fold higher HBV infection compared to the HepG2-NTCP-A3 parental clone. In addition, though HBV infectivity was universally reduced in the absence of polyethylene glycol (PEG), subclone C2 maintained relatively greater permissiveness under PEG-free conditions, suggesting the functional heterogeneity within parental HepG2-NTCP-A3 may be exploitable in developing a PEG-free HBV infection model. The increased viral production correlated with increased intracellular viral antigen expression as evidenced through HBcAg immunofluorescence staining. Further, these subclones were found to express different levels of NTCP, albeit with no remarkable morphology or cell growth differences. In conclusion, we isolated the subclones of HepG2-NTCP-A3 which support efficient HBV production and thus provide an improved in vitro HBV infection model. [ABSTRACT FROM AUTHOR]

Published

2022

8. Improved Plasmodium falciparum dilution cloning through efficient quantification of parasite numbers and c-SNARF detection

Author

Tatiane Macedo-Silva, Sanjay A. Desai, and Gerhard Wunderlich

Subjects

Malaria, Plasmodium, Cloning, Limiting dilution, Arctic medicine. Tropical medicine, RC955-962, Infectious and parasitic diseases, RC109-216

Abstract

Abstract Background Molecular and genetic studies of blood-stage Plasmodium falciparum parasites require limiting dilution cloning and prolonged cultivation in microplates. The entire process is laborious and subject to errors due to inaccurate dilutions at the onset and failed detection of parasite growth in individual microplate wells. Methods To precisely control the number of parasites dispensed into each microplate well, parasitaemia and total cell counts were determined by flow cytometry using parasite cultures stained with ethidium bromide or SYBR Green I. Microplates were seeded with 0.2 or 0.3 infected cells/well and cultivated with fresh erythrocytes. The c-SNARF fluorescent pH indicator was then used to reliably detect parasite growth. Results Flow cytometry required less time than the traditional approach of estimating parasitaemia and cell numbers by microscopic examination. The resulting dilutions matched predictions from Poisson distribution calculations and yielded clonal lines. Addition of c-SNARF to media permitted rapid detection of parasite growth in microplate wells with high confidence. Conclusion The combined use of flow cytometry for precise dilution and the c-SNARF method for detection of growth improves limiting dilution cloning of P. falciparum. This simple approach saves time, is scalable, and maximizes identification of desired parasite clones. It will facilitate DNA transfection studies and isolation of parasite clones from ex vivo blood samples.

Published

2021

9. Genetic barcoding reveals clonal dominance in iPSC-derived mesenchymal stromal cells

Author

Jonathan Hollmann, Johanna Brecht, Roman Goetzke, Julia Franzen, Anton Selich, Marco Schmidt, Monika Eipel, Alina Ostrowska, Jan Hapala, Eduardo Fernandez-Rebollo, Gerhard Müller-Newen, Michael Rothe, Thomas Eggermann, Martin Zenke, and Wolfgang Wagner

Subjects

Mesenchymal stromal cells, Induced pluripotent stem cells, Clonality, RGB marking, Genetic barcoding, Limiting dilution, Medicine (General), R5-920, Biochemistry, QD415-436

Abstract

Abstract Background The use of mesenchymal stromal cells (MSCs) for research and clinical application is hampered by cellular heterogeneity and replicative senescence. Generation of MSC-like cells from induced pluripotent stem cells (iPSCs) may circumvent these limitations, and such iPSC-derived MSCs (iMSCs) are already tested in clinical trials. So far, a comparison of MSCs and iMSCs was particularly addressed in bulk culture. Despite the high hopes in cellular therapy, only little is known how the composition of different subclones changes in these cell preparations during culture expansion. Methods In this study, we used multicolor lentiviral genetic barcoding for the marking of individual cells within cell preparations. Based on this, we could track the clonal composition of syngenic MSCs, iPSCs, and iMSCs during culture expansion. Furthermore, we analyzed DNA methylation patterns at senescence-associated genomic regions by barcoded bisulfite amplicon sequencing. The proliferation and differentiation capacities of individual subclones within MSCs and iMSCs were investigated with limiting dilution assays. Results Overall, the clonal composition of primary MSCs and iPSCs gradually declined during expansion. In contrast, iMSCs became oligoclonal early during differentiation, indicating that they were derived from few individual iPSCs. This dominant clonal outgrowth of iMSCs was not associated with changes in chromosomal copy number variation. Furthermore, clonal dynamics were not clearly reflected by stochastically acquired DNA methylation patterns. Limiting dilution assays revealed that iMSCs are heterogeneous in colony formation and in vitro differentiation potential, while this was even more pronounced in primary MSCs. Conclusions Our results indicate that the subclonal diversity of MSCs and iPSCs declines gradually during in vitro culture, whereas derivation of iMSCs may stem from few individual iPSCs. Differentiation regimen needs to be further optimized to achieve homogeneous differentiation of iPSCs towards iMSCs.

Published

2020

10. The Parasite Reduction Ratio (PRR) Assay Version 2: Standardized Assessment of Plasmodium falciparum Viability after Antimalarial Treatment In Vitro

Author

Annabelle Walz, Maëlle Duffey, Ghaith Aljayyoussi, Sibylle Sax, Didier Leroy, Dominique Besson, Jeremy N. Burrows, Mohammed H. Cherkaoui-Rbati, Nathalie Gobeau, Marie-Anne Westwood, Christoph Siethoff, Francisco-Javier Gamo, Pascal Mäser, and Sergio Wittlin

Subjects

malaria, Plasmodium falciparum, parasite viability, limiting dilution, parasite reduction ratio, PRR, Medicine, Pharmacy and materia medica, RS1-441

Abstract

With artemisinin-resistant Plasmodium falciparum parasites emerging in Africa, the need for new antimalarial chemotypes is persistently high. The ideal pharmacodynamic parameters of a candidate drug are a rapid onset of action and a fast rate of parasite killing or clearance. To determine these parameters, it is essential to discriminate viable from nonviable parasites, which is complicated by the fact that viable parasites can be metabolically inactive, whilst dying parasites can still be metabolically active and morphologically unaffected. Standard growth inhibition assays, read out via microscopy or [3H] hypoxanthine incorporation, cannot reliably discriminate between viable and nonviable parasites. Conversely, the in vitro parasite reduction ratio (PRR) assay is able to measure viable parasites with high sensitivity. It provides valuable pharmacodynamic parameters, such as PRR, 99.9% parasite clearance time (PCT99.9%) and lag phase. Here we report the development of the PRR assay version 2 (V2), which comes with a shorter assay duration, optimized quality controls and an objective, automated analysis pipeline that systematically estimates PRR, PCT99.9% and lag time and returns meaningful secondary parameters such as the maximal killing rate of a drug (Emax) at the assayed concentration. These parameters can be fed directly into pharmacokinetic/pharmacodynamic models, hence aiding and standardizing lead selection, optimization, and dose prediction.

Published

2023

11. A Bench-Top Approach for Isolation of Single Antibody Producing Chinese Hamster Ovary (CHO) Cells Using a Microwell-Based Microfluidic Device

Author

Salma Fuadiyah, Kittipat Chotchindakun, Rungrueang Phatthanakun, Panwong Kuntanawat, and Montarop Yamabhai

Subjects

monoclonal cell lines, cell line generation, single-cell cloning, limiting dilution, microfluidic device, Mechanical engineering and machinery, TJ1-1570

Abstract

Genetically-modified monoclonal cell lines are currently used for monoclonal antibody (mAbs) production and drug development. The isolation of single transformed cells is the main hindrance in the generation of monoclonal lines. Although the conventional limiting dilution method is time-consuming, laborious, and skill-intensive, high-end approaches such as fluorescence-activated cell sorting (FACS) are less accessible to general laboratories. Here, we report a bench-top approach for isolating single Chinese hamster ovary (CHO) cells using an adapted version of a simple microwell-based microfluidic (MBM) device previously reported by our group. After loading the cell suspension to the device, the electrostatically trapped cells can be viewed under a microscope and transferred using a micropipette for further clone establishment. Compared to the conventional method, the invented approach provided a 4.7-fold increase in the number of single cells isolated per round of cell loading and demonstrated a 1.9-fold decrease in total performing time. Additionally, the percentage of correct single-cell identifications was significantly improved, especially in novice testers, suggesting a reduced skill barrier in performing the task. This novel approach could serve as a simple, affordable, efficient, and less skill-intensive alternative to the conventional single-cell isolation for monoclonal cell line establishment.

Published

2022

12. Improved Plasmodium falciparum dilution cloning through efficient quantification of parasite numbers and c-SNARF detection.

Author

Macedo-Silva, Tatiane, Desai, Sanjay A., and Wunderlich, Gerhard

Subjects

*PLASMODIUM falciparum, *GENE transfection, *FLUORESCENT probes, *DILUTION, *MOLECULAR cloning, *BABESIA

Abstract

Background: Molecular and genetic studies of blood-stage Plasmodium falciparum parasites require limiting dilution cloning and prolonged cultivation in microplates. The entire process is laborious and subject to errors due to inaccurate dilutions at the onset and failed detection of parasite growth in individual microplate wells. Methods: To precisely control the number of parasites dispensed into each microplate well, parasitaemia and total cell counts were determined by flow cytometry using parasite cultures stained with ethidium bromide or SYBR Green I. Microplates were seeded with 0.2 or 0.3 infected cells/well and cultivated with fresh erythrocytes. The c-SNARF fluorescent pH indicator was then used to reliably detect parasite growth. Results: Flow cytometry required less time than the traditional approach of estimating parasitaemia and cell numbers by microscopic examination. The resulting dilutions matched predictions from Poisson distribution calculations and yielded clonal lines. Addition of c-SNARF to media permitted rapid detection of parasite growth in microplate wells with high confidence. Conclusion: The combined use of flow cytometry for precise dilution and the c-SNARF method for detection of growth improves limiting dilution cloning of P. falciparum. This simple approach saves time, is scalable, and maximizes identification of desired parasite clones. It will facilitate DNA transfection studies and isolation of parasite clones from ex vivo blood samples. [ABSTRACT FROM AUTHOR]

Published

2021

13. Investigation into limiting dilution and tick transmissibility phenotypes associated with attenuation of the S24 vaccine strain

Author

Ben J. Mans, Ronel Pienaar, P. Christo Troskie, and Michael P. Combrink

Subjects

Babesia bovis, Vaccine, Tick transmission, Limiting dilution, Sequestration, Genetic recombination, Infectious and parasitic diseases, RC109-216

Abstract

Abstract Background Babesia bovis is the causal agent of Asiatic redwater, transmitted by the pandemic tick Rhipicephalus (Boophilus) microplus. Disease control may target the tick vector using acaricides or anti-tick vaccines, or the parasite using chemoprophylaxis or anti-parasite vaccines. Current anti-parasite vaccines comprise live blood vaccines using attenuated B. bovis strains. Attenuation is attained by rapid passage that may result in different phenotypes such as reduced virulence, non-transmissibility by the tick vector, inability to sequester in the host (lack of limiting dilution) and limited genetic diversity. Attenuation and phenotypes may be linked to selection of subpopulations during rapid passage. The South African B. bovis S24 vaccine strain comprise a subpopulation that present low virulence, non-transmissibility, lack of limiting dilution phenotype and the presence of a single A558 Bv80 allele. The S24 strain could be co-transmitted with a field strain (05-100) suggesting sexual recombination. The present study investigated the change in phenotype for the S24 vaccine strain during rapid passage and co-transmission. Methods Vaccine phenotype change during passage as well as co-transmissibility was monitored using Bv80 allele specific PCR, limiting dilution and Illumina-based genome sequencing. Results The S24 population could not be rescued from the S16 passage as previously attained suggesting that selection of the S24 vaccine strain was a serendipitous and stochastic event. Passage from S16 to S24 also resulted in loss of the limiting dilution phenotype. Genome sequencing indicated sexual recombination during co-transmission with the 05-100 field strain. Analysis of the recombinant strain indicate that VESA1, smORF and SBP2 family members are present and may be responsible for the limiting dilution phenotypes, while various regions may also be responsible for the tick transmission phenotype. Conclusions The molecular basis for tick transmission and limiting dilution phenotypes may be defined in future using selection based on these traits in combination with sexual recombination.

Published

2019

14. Comparison of Two Strategies to Generate Antigen-Specific Human Monoclonal Antibodies: Which Method to Choose for Which Purpose?

Author

Anna M. Ehlers, Constance F. den Hartog Jager, Tineke Kardol-Hoefnagel, Miriam M.D. Katsburg, André C. Knulst, and Henny G. Otten

Subjects

monoclonal antibodies, single cell sequencing, immortalization, limiting dilution, antigen-specific B cells, Immunologic diseases. Allergy, RC581-607

Abstract

Human monoclonal antibodies (mAbs) are valuable tools to link genetic information with functional features and to provide a platform for conformational epitope mapping. Additionally, combined data on genetic and functional features provide a valuable mosaic for systems immunology approaches. Strategies to generate human mAbs from peripheral blood have been described and used in several studies including single cell sequencing of antigen-binding B cells and the establishment of antigen-specific monoclonal Epstein-Barr Virus (EBV) immortalized lymphoblastoid cell lines (LCLs). However, direct comparisons of these two strategies are scarce. Hence, we sought to set up these two strategies in our laboratory using peanut 2S albumins (allergens) and the autoantigen anti-Rho guanosine diphosphate dissociation inhibitor 2 (RhoGDI2, alternatively ‘ARHGDIB’) as antigen targets to directly compare these strategies regarding costs, time expenditure, recovery, throughput and complexity. Regarding single cell sequencing, up to 50% of corresponding V(D)J gene transcripts were successfully amplified of which 54% were successfully cloned into expression vectors used for heterologous expression. Seventy-five percent of heterologously expressed mAbs showed specific binding to peanut 2S albumins resulting in an overall recovery of 20.3%, which may be increased to around 29% by ordering gene sequences commercially for antibody cloning. In comparison, the establishment of monoclonal EBV-LCLs showed a lower overall recovery of around 17.6%. Heterologous expression of a mAb carrying the same variable region as its native counterpart showed comparable concentration-dependent binding abilities. By directly comparing those two strategies, single cell sequencing allows a broad examination of antigen-binding mAbs in a moderate-throughput manner, while the establishment of monoclonal EBV-LCLs is a powerful tool to select a small number of highly reactive mAbs restricted to certain B cell subpopulations. Overall, both strategies, initially set-up for peanut 2S albumins, are suitable to obtain human mAbs and they are easily transferrable to other target antigens as shown for ARHGDIB.

Published

2021

15. Comparison of Two Strategies to Generate Antigen-Specific Human Monoclonal Antibodies: Which Method to Choose for Which Purpose?

Author

Ehlers, Anna M., den Hartog Jager, Constance F., Kardol-Hoefnagel, Tineke, Katsburg, Miriam M.D., Knulst, André C., and Otten, Henny G.

Subjects

MONOCLONAL antibodies, LYMPHOBLASTOID cell lines, ANTIGENS, GENETIC vectors, B cells, ALBUMINS, LYMPHOCYTOSIS

Abstract

Human monoclonal antibodies (mAbs) are valuable tools to link genetic information with functional features and to provide a platform for conformational epitope mapping. Additionally, combined data on genetic and functional features provide a valuable mosaic for systems immunology approaches. Strategies to generate human mAbs from peripheral blood have been described and used in several studies including single cell sequencing of antigen-binding B cells and the establishment of antigen-specific monoclonal Epstein-Barr Virus (EBV) immortalized lymphoblastoid cell lines (LCLs). However, direct comparisons of these two strategies are scarce. Hence, we sought to set up these two strategies in our laboratory using peanut 2S albumins (allergens) and the autoantigen anti-Rho guanosine diphosphate dissociation inhibitor 2 (RhoGDI2, alternatively 'ARHGDIB') as antigen targets to directly compare these strategies regarding costs, time expenditure, recovery, throughput and complexity. Regarding single cell sequencing, up to 50% of corresponding V(D)J gene transcripts were successfully amplified of which 54% were successfully cloned into expression vectors used for heterologous expression. Seventy-five percent of heterologously expressed mAbs showed specific binding to peanut 2S albumins resulting in an overall recovery of 20.3%, which may be increased to around 29% by ordering gene sequences commercially for antibody cloning. In comparison, the establishment of monoclonal EBV-LCLs showed a lower overall recovery of around 17.6%. Heterologous expression of a mAb carrying the same variable region as its native counterpart showed comparable concentration-dependent binding abilities. By directly comparing those two strategies, single cell sequencing allows a broad examination of antigen-binding mAbs in a moderate-throughput manner, while the establishment of monoclonal EBV-LCLs is a powerful tool to select a small number of highly reactive mAbs restricted to certain B cell subpopulations. Overall, both strategies, initially set-up for peanut 2S albumins, are suitable to obtain human mAbs and they are easily transferrable to other target antigens as shown for ARHGDIB. [ABSTRACT FROM AUTHOR]

Published

2021

16. Japanese encephalitis virus: Biological clones from a clinical isolate quasispecies show differing neurovirulence in vitro and in a mouse model.

Author

Shu Pin Yu, Kien Chai Ong, Soon Hao Tan, Perera, David, and Kum Thong Wong

Subjects

*JAPANESE encephalitis viruses, *VIRAL antigens, *MICE, *VIRUS cloning

Abstract

The Japanese encephalitis virus (JEV), a leading cause of encephalitis, exists as quasispecies in clinical isolates. Using a limiting dilution method combined with immunohistochemistry to detect viral antigens, 10 biological clones were isolated and purified from a clinical JEV isolate (CNS138/9) derived from an autopsy brain. These biological clones were tested for neurovirulence in SK-N-MC and NIE-115 neuronal cells, and a 2-week-old, footpad-infected, JE mouse model. Nine clones were found to be neurovirulent; one clone neuroattenuated. Although further studies are needed to determine genotypic differences, if any, in these clones, the limiting dilution purification and neurovirulence testing methods described herein should be useful for phenotypic studies of quasispecies of neurotropic viruses in general, and JEV and other flaviviruses in particular. [ABSTRACT FROM AUTHOR]

Published

2020

17. A Few Key Historical Events in the Antibody Field: The Alacritous Antibody.

Author

Lefkovits, Ivan

Subjects

*CELL physiology, *CLONE cells, *IMMUNE system, *IMMUNOGLOBULINS, *CELL culture

Abstract

We have coined the term "alacrity" to describe the extraordinary diversity of B cell activation potentials, even among cells in a single B cell clone responding to a single antigen. The discovery of methodologies for B cell culture in limiting dilution allowed scientists to identify the source of cellular heterogeneity among cells of the immune system. Analyses of individual B cells set the stage for more detailed descriptions of the factors that diversify B cell functions, some of which will be expanded upon by partner articles in this B cell issue. [ABSTRACT FROM AUTHOR]

Published

2020

18. Serendipity: Reflections on Being Mentored by Dr. Peter Doherty.

Author

Topham, David J.

Subjects

*RESPIRATORY infections, *VIGNETTES, *INFLUENZA, *REFLECTIONS

Abstract

This is a semiautobiographical and scientific account of my time in the Doherty Laboratory from 1994 to 1999. It includes personal vignettes as well as discussion of how our work has impacted the fields of influenza, respiratory infections and immunity. I also point out the long-term impacts on my career. [ABSTRACT FROM AUTHOR]

Published

2020

19. Genetic barcoding reveals clonal dominance in iPSC-derived mesenchymal stromal cells.

Author

Hollmann, Jonathan, Brecht, Johanna, Goetzke, Roman, Franzen, Julia, Selich, Anton, Schmidt, Marco, Eipel, Monika, Ostrowska, Alina, Hapala, Jan, Fernandez-Rebollo, Eduardo, Müller-Newen, Gerhard, Rothe, Michael, Eggermann, Thomas, Zenke, Martin, and Wagner, Wolfgang

Subjects

*GENETIC barcoding, *STROMAL cells, *INDUCED pluripotent stem cells, *DNA methylation, *CELLULAR therapy, *PLURIPOTENT stem cells, *METHYLATION

Abstract

Background: The use of mesenchymal stromal cells (MSCs) for research and clinical application is hampered by cellular heterogeneity and replicative senescence. Generation of MSC-like cells from induced pluripotent stem cells (iPSCs) may circumvent these limitations, and such iPSC-derived MSCs (iMSCs) are already tested in clinical trials. So far, a comparison of MSCs and iMSCs was particularly addressed in bulk culture. Despite the high hopes in cellular therapy, only little is known how the composition of different subclones changes in these cell preparations during culture expansion. Methods: In this study, we used multicolor lentiviral genetic barcoding for the marking of individual cells within cell preparations. Based on this, we could track the clonal composition of syngenic MSCs, iPSCs, and iMSCs during culture expansion. Furthermore, we analyzed DNA methylation patterns at senescence-associated genomic regions by barcoded bisulfite amplicon sequencing. The proliferation and differentiation capacities of individual subclones within MSCs and iMSCs were investigated with limiting dilution assays. Results: Overall, the clonal composition of primary MSCs and iPSCs gradually declined during expansion. In contrast, iMSCs became oligoclonal early during differentiation, indicating that they were derived from few individual iPSCs. This dominant clonal outgrowth of iMSCs was not associated with changes in chromosomal copy number variation. Furthermore, clonal dynamics were not clearly reflected by stochastically acquired DNA methylation patterns. Limiting dilution assays revealed that iMSCs are heterogeneous in colony formation and in vitro differentiation potential, while this was even more pronounced in primary MSCs. Conclusions: Our results indicate that the subclonal diversity of MSCs and iPSCs declines gradually during in vitro culture, whereas derivation of iMSCs may stem from few individual iPSCs. Differentiation regimen needs to be further optimized to achieve homogeneous differentiation of iPSCs towards iMSCs. [ABSTRACT FROM AUTHOR]

Published

2020

20. TLR9 Signaling Suppresses the Canonical Plasma Cell Differentiation Program in Follicular B Cells

Author

Bárbara José Antunes Baptista, Alessandra Granato, Fábio B. Canto, Fabricio Montalvão, Lucas Tostes, Herbert L. de Matos Guedes, Antonio Coutinho, Maria Bellio, Andre M. Vale, and Alberto Nobrega

Subjects

follicular B cell, plasma cell, TLR9, TLR4, limiting dilution, Immunologic diseases. Allergy, RC581-607

Abstract

The relative potency and quality of mouse B cell response to Toll-like receptors (TLRs) signaling varies significantly depending on the B cell subset and on the TLR member being engaged. Although it has been shown that marginal zone cells respond faster than follicular (FO) splenic B cells to TLR4 stimulus, FO B cells retain full capacity to proliferate and generate plasmablasts and plasma cells (PBs/PCs) with 2–3 days delayed kinetics. It is not clear whether this scenario could be extended to other members of the TLR family. Here, using quantitative cell culture conditions optimized for B cell growth and differentiation, we show that TLR9 signaling by CpG, while promoting vigorous proliferation, completely fails to induce differentiation of FO B cells into PBs/PCs. Little or absent Ig secretion following TLR9 stimulus was accompanied by lack of expression of cell surface markers and canonical transcription factors involved in PB/PC differentiation. Moreover, not only TLR9 did not induce plasmocyte differentiation, but it also strongly inhibited the massive PB/PC differentiation of FO B cells triggered by LPS/TLR4. Our study reveals unexpected opposite roles for TLR4 and TLR9 in the control of plasma cell differentiation program and disagrees with previous conclusions obtained in high-density cultures conditions on the generation of plasmocytes by TRL9 signaling. The potential implications of these findings on the role of TLR9 in controlling self-tolerance, clonal sizes and regulation of humoral responses are discussed.

Published

2018

21. Effects of hypoxic storage on the efficacy of gamma irradiation in abrogating lymphocyte proliferation and on the quality of gamma‐irradiated red blood cells in additive solution 3

Author

Samuel O. Sowemimo-Coker and Loren D. Fast

Subjects

Erythrocytes, Red Cell, Chemistry, Immunology, Hematology, Lymphocyte proliferation, Hypoxia (medical), Peripheral blood mononuclear cell, In vitro, Andrology, Blood Preservation, Gamma Rays, Limiting dilution, Leukocytes, Mononuclear, medicine, Humans, Immunology and Allergy, Irradiation, medicine.symptom, Hypoxia, Cell Proliferation, Gamma irradiation

Abstract

BACKGROUND Gamma irradiation of blood products is used to prevent transfusion-associated graft-versus-host disease by inhibiting the proliferation of lymphocytes that are implicated in the disease. Gamma irradiation also damages the red blood cells (RBCs). It is unknown whether hypoxia reduces the efficacy of gamma irradiation in inhibiting lymphocyte proliferation (LP). The objectives of the study were to investigate the effects of hypoxia on gamma irradiation-induced inhibition of LP and on the in vitro properties of RBCs. MATERIALS AND METHODS Forty-four units (300-340 ml each) of less than 8-h-old ABO-matched leukocyte reduced red cell concentrates (LR-RCC) in additive solution 3 were pooled in pairs. Peripheral blood mononuclear cells were isolated from non-leukocyte reduced RCCs and added back to the pool at a final concentration of 2 × 105 /ml. The pool was divided equally into a conventional storage bag A and a hypoxic processing and storage bag B. The units were gamma-irradiated at 25Gy on day 7 for the LP experiment and on either day 7 or 14 for the RBC quality experiments. LP was measured using a limiting dilution assay, and several in vitro metrics of RBCs were measured. RESULTS Gamma irradiation inhibited T-lymphocyte proliferation by 4.7 × 104 -fold reduction in both hypoxic and conventional storage. The in vitro metrics of RBC quality were better preserved in hypoxic storage. DISCUSSION T lymphocytes present in hypoxic RBC are equally susceptible to gamma irradiation as conventional storage. Hypoxic storage also reduces the deleterious effects of gamma irradiation on RBCs.

Published

2021

22. Technologies for Single-Cell Isolation

Author

Andre Gross, Jonas Schoendube, Stefan Zimmermann, Maximilian Steeb, Roland Zengerle, and Peter Koltay

Subjects

single-cell analysis, single-cell handling, single-cell separation, single-cell technologies, flow cytometry, laser microdissection, limiting dilution, microfluidics, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

The handling of single cells is of great importance in applications such as cell line development or single-cell analysis, e.g., for cancer research or for emerging diagnostic methods. This review provides an overview of technologies that are currently used or in development to isolate single cells for subsequent single-cell analysis. Data from a dedicated online market survey conducted to identify the most relevant technologies, presented here for the first time, shows that FACS (fluorescence activated cell sorting) respectively Flow cytometry (33% usage), laser microdissection (17%), manual cell picking (17%), random seeding/dilution (15%), and microfluidics/lab-on-a-chip devices (12%) are currently the most frequently used technologies. These most prominent technologies are described in detail and key performance factors are discussed. The survey data indicates a further increasing interest in single-cell isolation tools for the coming years. Additionally, a worldwide patent search was performed to screen for emerging technologies that might become relevant in the future. In total 179 patents were found, out of which 25 were evaluated by screening the title and abstract to be relevant to the field.

Published

2015

23. TLR9 Signaling Suppresses the Canonical Plasma Cell Differentiation Program in Follicular B Cells.

Author

Baptista, Bárbara José Antunes, Granato, Alessandra, Canto, Fábio B., Montalvão, Fabricio, Tostes, Lucas, de Matos Guedes, Herbert L., Coutinho, Antonio, Bellio, Maria, Vale, Andre M., and Nobrega, Alberto

Abstract

The relative potency and quality of mouse B cell response to Toll-like receptors (TLRs) signaling varies significantly depending on the B cell subset and on the TLR member being engaged. Although it has been shown that marginal zone cells respond faster than follicular (FO) splenic B cells to TLR4 stimulus, FO B cells retain full capacity to proliferate and generate plasmablasts and plasma cells (PBs/PCs) with 2–3 days delayed kinetics. It is not clear whether this scenario could be extended to other members of the TLR family. Here, using quantitative cell culture conditions optimized for B cell growth and differentiation, we show that TLR9 signaling by CpG, while promoting vigorous proliferation, completely fails to induce differentiation of FO B cells into PBs/PCs. Little or absent Ig secretion following TLR9 stimulus was accompanied by lack of expression of cell surface markers and canonical transcription factors involved in PB/PC differentiation. Moreover, not only TLR9 did not induce plasmocyte differentiation, but it also strongly inhibited the massive PB/PC differentiation of FO B cells triggered by LPS/TLR4. Our study reveals unexpected opposite roles for TLR4 and TLR9 in the control of plasma cell differentiation program and disagrees with previous conclusions obtained in high-density cultures conditions on the generation of plasmocytes by TRL9 signaling. The potential implications of these findings on the role of TLR9 in controlling self-tolerance, clonal sizes and regulation of humoral responses are discussed. [ABSTRACT FROM AUTHOR]

Published

2018

24. Functional assessment of spermatogonial stem cell purity in experimental cell populations.

Author

Lord, Tessa and Oatley, Jon M.

Abstract

Historically, research in spermatogonial biology has been hindered by a lack of validated approaches to identify and isolate pure populations of the various spermatogonial subsets for in-depth analysis. In particular, although a number of markers of the undifferentiated spermatogonial population have now been characterized, standardized methodology for assessing their specificity to the spermatogonial stem cell (SSC) and transit amplifying progenitor pools has been lacking. To date, SSC content within an undefined population of spermatogonia has been inferred using either lineage tracing or spermatogonial transplantation analyses which generate qualitative and quantitative data, respectively. Therefore, these techniques are not directly comparable, and are subject to variable interpretations as to a readout that is representative of a ‘pure’ SSC population. We propose standardization across the field for determining the SSC purity of a population via use of a limiting dilution transplantation assay that would eliminate subjectivity and help to minimize the generation of inconsistent data on ‘SSC’ populations. In the limiting dilution transplantation assay, a population of LacZ -expressing spermatogonia are selected based on a putative SSC marker, and a small, defined number of cells (i.e. 10 cells) are microinjected into the testis of a germ cell-deficient recipient mouse. Using colony counts and an estimated colonization efficiency of 5%; a quantitative value can be calculated that represents SSC purity in the starting population. The utilization of this technique would not only be useful to link functional relevance to novel markers that will be identified in the future, but also for providing validation of purity for marker-selected populations of spermatogonia that are commonly considered to be SSCs by many researchers in the field of spermatogenesis and stem cell biology. [ABSTRACT FROM AUTHOR]

Published

2018

25. Beating the odds: The poisson distribution of all input cells during limiting dilution grossly underestimates whether a cell line is clonally‐derived or not.

Author

Zhou, Yizhou, Shaw, David, Lam, Cynthia, Tsukuda, Joni, Yim, Mandy, Tang, Danming, Louie, Salina, Laird, Michael W., Snedecor, Brad, and Misaghi, Shahram

Subjects

POISSON distribution, CLONE cells, CELL lines, PROGENITOR cells, CLONING

Abstract

Establishing that a cell line was derived from a single cell progenitor and defined as clonally‐derived for the production of clinical and commercial therapeutic protein drugs has been the subject of increased emphasis in cell line development (CLD). Several regulatory agencies have expressed that the prospective probability of clonality for CHO cell lines is assumed to follow the Poisson distribution based on the input cell count. The probability of obtaining monoclonal progenitors based on the Poisson distribution of all cells suggests that one round of limiting dilution may not be sufficient to assure the resulting cell lines are clonally‐derived. We experimentally analyzed clonal derivatives originating from single cell cloning (SCC) via one round of limiting dilution, following our standard legacy cell line development practice. Two cell populations with stably integrated DNA spacers were mixed and subjected to SCC via limiting dilution. Cells were cultured in the presence of selection agent, screened, and ranked based on product titer. Post‐SCC, the growing cell lines were screened by PCR analysis for the presence of identifying spacers. We observed that the percentage of nonclonal populations was below 9%, which is considerably lower than the determined probability based on the Poisson distribution of all cells. These results were further confirmed using fluorescence imaging of clonal derivatives originating from SCC via limiting dilution of mixed cell populations expressing GFP or RFP. Our results demonstrate that in the presence of selection agent, the Poisson distribution of all cells clearly underestimates the probability of obtaining clonally‐derived cell lines. © 2017 American Institute of Chemical Engineers Biotechnol. Prog., 34:559–569, 2018 [ABSTRACT FROM AUTHOR]

Published

2018

26. Chapter One - Single-Cell Resolution of T Cell Immune Responses.

Author

Buchholz, Veit R. and Flossdorf, Michael

Subjects

ANTIGENS, T cells, B cells, IMMUNE response

Abstract

Single antigen-specific B or T lymphocytes are the smallest functional units, into which an adaptive immune response can be dissected. Today, novel high-throughput technologies are providing researches with increasingly complex information on the diverse phenotypic signatures of individual lymphocytes. With a focus on T cells, we summarize here, how computational approaches are becoming increasingly important to identify the relevant developmental boundaries and connections between these high-dimensional lymphocyte states. We then describe how these insights may be further expanded by novel experimental approaches that allow to map the fate of individual T cells and their progeny in vivo and in vitro. Finally, we highlight how these experiments have uncovered a probabilistic regulatory structure of T cell immune responses and briefly discuss, how two distinct theoretical frameworks used to describe this structure may be merged to best capture single T cell behavior in computational terms. [ABSTRACT FROM AUTHOR]

Published

2018

27. Improved Plasmodium falciparum dilution cloning through efficient quantification of parasite numbers and c-SNARF detection

Author

Gerhard Wunderlich, Tatiane Macedo-Silva, and Sanjay A. Desai

Subjects

0301 basic medicine, Microplate Well, Plasmodium, Dilution cloning, Serial dilution, ANIMAIS PARASITOS, medicine.medical_treatment, Plasmodium falciparum, 030231 tropical medicine, RC955-962, Naphthols, Infectious and parasitic diseases, RC109-216, Flow cytometry, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Limiting dilution, Arctic medicine. Tropical medicine, medicine, Parasite hosting, Benzopyrans, Cloning, Molecular, Malaria, Falciparum, medicine.diagnostic_test, biology, Rhodamines, Methodology, Flow Cytometry, biology.organism_classification, Molecular biology, Malaria, 030104 developmental biology, Infectious Diseases, chemistry, SYBR Green I, Parasitology, Ethidium bromide, Cloning

Abstract

Background Molecular and genetic studies of blood-stage Plasmodium falciparum parasites require limiting dilution cloning and prolonged cultivation in microplates. The entire process is laborious and subject to errors due to inaccurate dilutions at the onset and failed detection of parasite growth in individual microplate wells. Methods To precisely control the number of parasites dispensed into each microplate well, parasitaemia and total cell counts were determined by flow cytometry using parasite cultures stained with ethidium bromide or SYBR Green I. Microplates were seeded with 0.2 or 0.3 infected cells/well and cultivated with fresh erythrocytes. The c-SNARF fluorescent pH indicator was then used to reliably detect parasite growth. Results Flow cytometry required less time than the traditional approach of estimating parasitaemia and cell numbers by microscopic examination. The resulting dilutions matched predictions from Poisson distribution calculations and yielded clonal lines. Addition of c-SNARF to media permitted rapid detection of parasite growth in microplate wells with high confidence. Conclusion The combined use of flow cytometry for precise dilution and the c-SNARF method for detection of growth improves limiting dilution cloning of P. falciparum. This simple approach saves time, is scalable, and maximizes identification of desired parasite clones. It will facilitate DNA transfection studies and isolation of parasite clones from ex vivo blood samples.

Published

2021

28. Expression and purification of a major allergen, Pla a 1, from Platanus acerifolia pollen and the preparation of its monoclonal antibody.

Author

WEI‑WEI NI, WEN HUANG, DE‑QIN WU, YAN‑JUN ZHOU, CHUN‑MEI JI, MENG‑DA CAO, MIAO GUO, JIN‑LU SUN, and JI‑FU WEI

Subjects

*ALLERGENS, *SYCAMORES, *MONOCLONAL antibodies, *AIRBORNE infection, *HYBRIDOMAS, *ESCHERICHIA coli, *LABORATORY mice

Abstract

Platanus acerifolia pollen is considered an important source of airborne allergens in numerous cities. Pla a 1 is a major allergen from P. acerifolia pollen. The present study aimed to express and purify Pla a 1, and to prepare its monoclonal antibody. In the present study, the Pla a 1 gene was subcloned into a pET‑28a vector and transformed into the ArcticExpress™ (DE3) RP Escherichia coli host strain. The purified Pla a 1 was then used to immunize BALB/c mice. When serum detection was positive, spleen cells were isolated from the mice and fused with SP2/0 myeloma cells at a ratio of 10:1. Hybridoma cells were screened by indirect ELISA and limiting dilution. Positive cells were used to induce the formation of antibody‑containing ascites fluid, and the antibodies were purified using protein A‑agarose. The results of the present study demonstrated that recombinant Pla a 1 was successfully expressed and purified, and exhibited positive immunoglobulin E‑binding to serum from patients allergic to P. acerifolia. A total of 11 hybridomas that steadily secreted anti‑Pla a 1 antibody were obtained and an immunoblotting analysis indicated that all of these monoclonal antibodies specifically recognized the Pla a 1 protein. These results suggested that specific anti‑Pla a 1 antibodies may be obtained, which can be used for the rapid detection of Pla a 1 allergens and in the preparation of vaccines against P. acerifolia pollen. [ABSTRACT FROM AUTHOR]

Published

2017

29. Development and characterization of monoclonal antibody against human IL-37b.

Author

Gao, Yu-Chi, Jia, Yan, Xiao, De-Qian, Wang, Xin, Dai, You-Chao, Yu, Shi-Yan, Chen, Chen, Zhuang, Ze-Gang, Fu, Xiao-Xia, Zhang, Jun-Ai, Zheng, Bi-Ying, Chen, Zhi-Hong, Zhong, Ji-Xin, Chen, Zhang-Quan, and Xu, Jun-Fa

Abstract

IL-37 has been described as a natural inhibitor of immune responses. Monoclonal antibody (mAb) against human IL-37b with high affinity and specificity can serve as a molecular probe to detect IL-37 and study IL-37 functions, mechanisms and related signal pathways in inflammatory diseases. However, there are very few such mAbs against human IL-37 commercially available so far. In the current study, monoclonal antibodies against human IL-37b were developed by fusing splenocytes from immunized mouse with SP2/0 myeloma cells and polyethylene glycol. Then the antibodies were screened with prokaryotic expressed human IL-37b protein and eukaryotic expressed human IL-37b protein subsequently. Western blot and flow cytometry analysis revealed that selected mAb clons were able to recognize human IL-37 with high specificity. And more importantly, the IL-37b mAbs were fluorescently labeled and can be directly used in flow cytometry and immunohistochemistry. In conclusion, the current study developed new mAbs against human IL-37b, which are applicable in flow cytometry and immunohistochemistry. [ABSTRACT FROM AUTHOR]

Published

2017

30. Serendipity: Reflections on Being Mentored by Dr. Peter Doherty

Author

David J. Topham

Subjects

0301 basic medicine, Biomedical Research, Psychoanalysis, Serendipity, Mentors, Immunology, T cell, immunity, Education, limiting dilution, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, Allergy and Immunology, Virology, Limiting dilution, Influenza, Human, parainfluenza, Humans, Molecular Medicine, 030211 gastroenterology & hepatology, influenza, Psychology, Respiratory Tract Infections, Personal Reflections

Abstract

This is a semiautobiographical and scientific account of my time in the Doherty Laboratory from 1994 to 1999. It includes personal vignettes as well as discussion of how our work has impacted the fields of influenza, respiratory infections and immunity. I also point out the long-term impacts on my career.

Published

2020

31. Characterization of Persistent Infection of Megalocytivirus in PMF Cell Line Derived from the Fin of Red Sea Bream Pagrus major

Author

Hyun-Do Jeong, Min-Gyeong Jeong, Joon-Gyu Min, and Woo-Ju Kwon

Subjects

Pagrus major, Fin, Cell culture, Limiting dilution, Biology, Megalocytivirus, biology.organism_classification, Molecular biology

Published

2019

32. Long-term culture-initiating cells (LTC-IC) produced from CD34+ cord blood cells with limiting dilution method

Author

Gülderen Yanıkkaya Demirel, Tülin Budak-Alpdoğan, Sema Aktaş, and Mahmut Bayık

Subjects

Stem cell, cord blood, LTC-IC, limiting dilution, CFU assay, cytometry, Diseases of the blood and blood-forming organs, RC633-647.5

Abstract

Objective: Even though much progress has been made in defining primitive hematologic cell phenotypes by using flow cytometry and clonogenic methods, the direct method for study of marrow repopulating cells still remains to be elusive. Long Term Culture-Initiating Cells (LTC-IC) are known as the most primitive human hematopoietic cells detectable by in vitro functional assays. Materials and Methods: In this study, LTC-IC with limiting dilution assay was used to evaluate repopulating potential of cord blood stem cells. Results: CD34 selections from cord blood were completed succesfully with magnetic beads (73,64%±9,12). The average incidence of week 5 LTC-IC was 1: 1966 CD34+ cells (range 1261–2906).Conclusion: We found that number of LTC-IC obtained from CD34+ cord blood cells were relatively low in numbers when compared to previously reported bone marrow CD34+ cells. This may be due to the lack of some transcription and growth factors along with some cytokines and chemokines released by accessory cells which are necessary for proliferation of cord blood progenitor/stem cells and it presents an area of interest for further studies.

Published

2010

33. Long-term effects of early antiretroviral initiation on HIV reservoir markers: a longitudinal analysis of the MERLIN clinical study

Author

Trupti Gilada, Jessica Rios, Nicolas Chomont, Marta Massanella, Ricardo Alfaro, Amélie Pagliuzza, Carmela Ganoza, Ann Duerr, Javier R. Lama, Rachel A Bender Ignacio, Delia M. Pinto-Santini, and Sayan Dasgupta

Subjects

Microbiology (medical), Adult, Male, medicine.medical_specialty, Medicine (General), Canada, Adolescent, Art initiation, Human immunodeficiency virus (HIV), HIV Infections, medicine.disease_cause, Microbiology, Transgender women, Article, Men who have sex with men, Clinical study, Sexual and Gender Minorities, Young Adult, R5-920, Virology, Internal medicine, Limiting dilution, medicine, Humans, Homosexuality, Male, Neurofibromin 2, business.industry, Middle Aged, Antiretroviral therapy, QR1-502, United States, Infectious Diseases, Anti-Retroviral Agents, DNA, Viral, HIV-1, Leukocytes, Mononuclear, Female, business, Viral load, Biomarkers

Abstract

Summary Background Early antiretroviral therapy (ART) initiation (ie, within 3 months of infection) limits establishment of the HIV reservoir. However, the effect of early ART initiation on the long-term dynamics of the pool of infected cells remains unclear. Methods In this longitudinal analysis, we included cisgender men who have sex with men (MSM) and transgender women (aged 18–54 years) at high risk for HIV infection, enrolled in the ongoing longitudinal MERLIN study in Peru between Oct 28, 2014, and Nov 8, 2018. Participants were eligible if they had been infected with HIV less than 90 days before enrolment, and if they had cryopreserved peripheral blood mononuclear cell (PBMC) samples. Participants were stratified into three groups on the basis of whether they initiated ART at 30 days or less (acute group), at 31–90 days (early group), or more than 24 weeks (deferred group) after the estimated date of detectable infection. PBMC samples were collected before ART initiation and longitudinally for up to 4 years on ART. The main outcomes were to establish the size of the HIV reservoir before ART initiation and to assess the effect of the timing of ART initiation on the decay of the HIV reservoir over 4 years follow-up. We quantified viral load, and isolated CD4 cells to quantify total HIV DNA, integrated HIV DNA and 2-long terminal repeat circles. Longitudinal analysis of active and inducible HIV reservoirs were measured by quantifying the frequency of CD4 cells producing multiply-spliced HIV RNA ex vivo and after in-vitro stimulation with a tat/rev induced limiting dilution assay (TILDA). A mixed-effects model from the time of ART initiation was used to measure longitudinal decays in viral loads and each HIV reservoir measure in each of the three groups. Findings We included 56 participants in this analysis, all of whom were MSM: 15 were in the acute group, 19 were in the early group, and 22 were in the deferred group. Participants in all three groups had similar levels of all HIV reservoir markers before ART initiation. All participants, including those in the acute group, had a pool of transcriptionally silent HIV-infected cells before ART initiation, as indicated by a substantial increase in TILDA measures upon stimulation. Longitudinal analysis over 4 years of ART revealed a biphasic decay of all HIV persistence markers, with a rapid initial decline followed by a slower decay in all participants. During the first-phase decay, the half-lives of both total and integrated HIV DNA and TILDA measures were significantly shorter in the acute group than in the early and deferred groups. During the second-phase decay, HIV reservoir markers continued to decline only in participants in the acute group. Interpretation Participants who initiated ART within 30 days or less of HIV infection showed a steeper and more sustained decay in HIV reservoir measures, suggesting long-term benefit of acute ART initiation on reservoir clearance. Funding The US National Institutes of Health and the Canadian Institutes for Health Research.

Published

2021

34. An Improved Tat/Rev Induced Limiting Dilution Assay With Enhanced Sensitivity and Breadth of Detection

Author

Swarnima Mishra, G. N. Sanjeeva, Afzal Amanullah, Narendra Nala, Anish D’silva, Deepak Selvam, Udaykumar Ranga, Kavita Mehta, Yuvrajsinh Gohil, and Neelam Pargain

Subjects

0301 basic medicine, Immunology, HIV Infections, Polymerase Chain Reaction, Sensitivity and Specificity, Cell Line, 03 medical and health sciences, 0302 clinical medicine, Limiting dilution, Methods, Humans, Immunology and Allergy, Enhanced sensitivity, Conserved Sequence, Chemistry, transcriptional silence, Genetic Variation, Reproducibility of Results, latent reservoir, rev Gene Products, Human Immunodeficiency Virus, Viral Load, RC581-607, Molecular biology, Virus Latency, 030104 developmental biology, HIV-1, RNA, Viral, tat Gene Products, Human Immunodeficiency Virus, TILDA, Immunologic diseases. Allergy, HIV latency, Nucleic Acid Amplification Techniques, 030217 neurology & neurosurgery

Abstract

Tat/Rev Induced Limiting Dilution Assay (TILDA) is instrumental in estimating the size of latent reservoirs of HIV-1. Here, we report an optimized TILDA containing a broader detection range compared to the reported methods and high sensitivity. Giving priority to sequence conservation, we positioned the two forward primers and the probe in exon-1 of HIV-1. The reverse primers are positioned in highly conserved regions of exon-7. The optimized TILDA detected eight molecular clones belonging to five major genetic subtypes of HIV-1 with a comparable detection sensitivity. Using the optimized assay, we show that only a minor proportion of CD4+ T cells of primary clinical samples can spontaneously generate multiply spliced viral transcripts. A significantly larger proportion of the cells produced viral transcripts following activation. The optimized TILDA is suitable to characterize HIV-1 latent reservoirs and the therapeutic strategies intended to target the reservoir size.

Published

2021

35. Microfluidic chip-based single-cell cloning to accelerate biologic production timelines

Author

Kim Le, Ewelina Zasadzinska, Jennitte Stevens, Natalia Gomez, Jasmine Tat, Ryan Zastrow, Huong Le, Jonathan Diep, and Pheng Yam

Subjects

Cloning, Recombinant Fusion Proteins, Timeline, Computational biology, CHO Cells, Biology, Cell sorting, Microfluidic Analytical Techniques, Flow Cytometry, Speed to market, Cricetulus, Microfluidic chip, Limiting dilution, Cricetinae, Immunoglobulin G, Lab-On-A-Chip Devices, Animals, Humans, Biomanufacturing, Cloning, Molecular, Single-Cell Analysis, Population doubling, Biotechnology

Abstract

Cell line development (CLD) represents a critical, yet time-consuming, step in the biomanufacturing process as significant resources are devoted to the scale-up and screening of several hundreds to thousands of single-cell clones. Typically, transfected pools are fully recovered from selection and characterized for growth, productivity, and product quality to identify the best pools suitable for single-cell cloning (SCC) using limiting dilution or fluorescence-activated cell sorting (FACS). Here we report the application of the Berkeley Lights Beacon Instrument (BLI) in an early SCC process to accelerate the CLD timeline. Transfected pools were single-cell cloned when viabilities reached greater than 85% or during selection when viabilities were less than 30%. Clones isolated from these accelerated processes exhibited comparable growth, productivity, and product quality to those derived from a standard CLD process and fit into an existing manufacturing platform. With these approaches, up to a 30% reduction in the overall CLD timeline was achieved. Furthermore, early process-derived clones demonstrated equivalent long-term stability compared with standard process-derived clones over 50 population doubling levels (PDLs). Taken together, the data supported early SCC on the BLI as an attractive approach to reducing the standard CLD timeline while still identifying clones with acceptable manufacturability.

Published

2021

36. A Tat/Rev Induced Limiting Dilution Assay to Measure Viral Reservoirs in Non-Human Primate Models of HIV Infection

Author

Ines Frank, Arpan Acharya, Svetlana Mazel, Stanka Semova, Meropi Aravantinou, Nanda Kishore Routhu, Elena Martinelli, Maria Sole Cigoli, Siddappa N. Byrareddy, Stephanie Maldonado, Mirko Paiardini, Justin L. Harper, and Nina Derby

Subjects

CD4-Positive T-Lymphocytes, Primates, 0301 basic medicine, viruses, Simian Acquired Immunodeficiency Syndrome, lcsh:Medicine, HIV Infections, Stimulation, Viremia, Biology, Virus Replication, Article, 03 medical and health sciences, 0302 clinical medicine, Limiting dilution, medicine, Animals, Humans, lcsh:Science, Multidisciplinary, Macrophages, lcsh:R, RNA, virus diseases, rev Gene Products, Human Immunodeficiency Virus, Viral Load, medicine.disease, Macaca mulatta, Virology, In vitro, Virus Latency, 3. Good health, Experimental models of disease, Disease Models, Animal, 030104 developmental biology, Viral replication, Preclinical research, Cell culture, HIV-1, RNA, Viral, Simian Immunodeficiency Virus, tat Gene Products, Human Immunodeficiency Virus, lcsh:Q, Lymph, Infection, 030217 neurology & neurosurgery

Abstract

The establishment of latent infection and poorly characterized viral reservoirs in tissues represent major obstacles to a definitive cure for HIV. Non-human primate (NHP) models of HIV infection are critical to elucidate pathogenic processes and an essential tool to test novel therapeutic strategies. Thus, the availability of novel assays to measure residual viral replication and reservoirs in NHP models may increase their utility in the search for an HIV cure. We developed a tat/rev induced limiting dilution assay to measure the frequency of CD4+ T cells that express multiply-spliced(ms)_SIV RNA in presence and absence of stimulation. We validated the assay using cell lines and cells from blood and lymph nodes of SIV infected macaques. In vitro, SIV/SHIV TILDA detects only cells expressing viral proteins. In SIV/SHIV-infected macaques, CD4+ T cells that express msSIV/SHIV RNA (TILDA data) were detected also in the setting of very low/undetectable viremia. TILDA data were significantly higher after stimulation and correlated with plasma viral load (pVL). Interestingly, TILDA data from early cART initiation correlated with peak and AUC pVL post-cART interruption. In summary, we developed an assay that may be useful in characterizing viral reservoirs and determining the effect of HIV interventions in NHP models.

Published

2019

37. Inducible HIV-1 Reservoir Quantification: Clinical Relevance, Applications and Advancements of TILDA

Author

Cynthia Lungu, Francesco A. Procopio, Riddhima Banga, Rob A. Gruters, and Virology

Subjects

Microbiology (medical), Computer science, HIV-1 cure, Human immunodeficiency virus (HIV), Computational biology, medicine.disease_cause, Microbiology, Hiv 1 latency, 03 medical and health sciences, SDG 3 - Good Health and Well-being, Limiting dilution, medicine, Clinical significance, 030304 developmental biology, Alternative methods, reservoir quantification, 0303 health sciences, 030306 microbiology, Gold standard (test), Provirus, QR1-502, 3. Good health, Perspective, HIV-1 latency, inducible reservoir, TILDA

Abstract

The presence of a stable HIV-1 reservoir persisting over time despite effective antiretroviral suppression therapy precludes a cure for HIV-1. Characterizing and quantifying this residual reservoir is considered an essential prerequisite to develop and validate curative strategies. However, a sensitive, reproducible, cost-effective, and easily executable test is still needed. The quantitative viral outgrowth assay is considered the gold standard approach to quantify the reservoir in HIV-1-infected patients on suppressive ART, but it has several limitations. An alternative method to quantify the viral reservoir following the reactivation of latent HIV-1 provirus detects multiply-spliced tat/rev RNA (msRNA) molecules by real-time PCR [tat/rev induced limiting dilution assay (TILDA)]. This article provides a perspective overview of the clinical relevance, various applications, recent advancements of TILDA, and how the assay has contributed to our understanding of the HIV-1 reservoir.

Published

2021

38. Analysis of The Cells Isolated From Epithelial Cell Rests of Malassez Through Single-cell Limiting Dilution

Author

Sakakibara S, Kurashige Y, Abiko Y, Bolortsetseg D, Saitoh M, Okada Y, Minowa E, and Islam St

Subjects

medicine.anatomical_structure, genetic structures, stomatognathic system, Chemistry, Limiting dilution, Cell, medicine, Epithelial cell rests of Malassez, biochemical phenomena, metabolism, and nutrition, Cell biology

Abstract

The epithelial cell rests of Malassez (ERM) play a pivotal role in preventing ankylosis between the alveolar bone and the tooth. Although several functions of ERM has been reported, the mechanism behind preventing dentoalveolar ankylosis remains unclear. In this study, 18 clones were isolated from ERM (CRUDE) using the single-cell limiting dilution method. Among them, ERM-2 and -3, which exhibited the highest and lowest proliferation rates, respectively, were selected. ERM-2, ERM-3, and CRUDE ERM were stained with epithelial markers, including cytokeratin-wide and cytokeratin-19, via immunofluorescence. The qRT-PCR analysis revealed increased expression levels of p75 (ameloblast marker), amelogenin, and sfrp5 (inner enamel epithelial cell marker) in the ERM-2 cells. Alternatively, ameloblastin and ck-14 (outer enamel epithelial cell marker) were highly expressed in ERM-3 cells. The mineralization of human periodontal ligament fibroblast (HPDLF) was inhibited when co-cultured with ERM-2, ERM-3, and CRUDE ERM cells. The addition of an anti-amelogenin antibody restored the mineralization of HPDLF cells. Transplanted rat molar cultured in ERM-2 (high amelogenin secretive clone) cell-derived supernatant resulted in significantly smaller bone formation than those cultured in the CRUDE ERM and ERM-3 cell-derived supernatants. These findings indicate that amelogenin produced by ERM cells might be involved in preventing dentoalveolar ankylosis.

Published

2021

39. Technologies for Single-Cell Isolation.

Author

Gross, Andre, Schoendube, Jonas, Zimmermann, Stefan, Steeb, Maximilian, Zengerle, Roland, and Koltay, Peter

Subjects

*CELL separation, *CYTOPROTECTION, *CYTOLOGY, *CYTOMETRY, *CANCER research

Abstract

The handling of single cells is of great importance in applications such as cell line development or single-cell analysis, e.g., for cancer research or for emerging diagnostic methods. This review provides an overview of technologies that are currently used or in development to isolate single cells for subsequent single-cell analysis. Data from a dedicated online market survey conducted to identify the most relevant technologies, presented here for the first time, shows that FACS (fluorescence activated cell sorting) respectively Flow cytometry (33% usage), laser microdissection (17%), manual cell picking (17%), random seeding/dilution (15%), and microfluidics/lab-on-a-chip devices (12%) are currently the most frequently used technologies. These most prominent technologies are described in detail and key performance factors are discussed. The survey data indicates a further increasing interest in single-cell isolation tools for the coming years. Additionally, a worldwide patent search was performed to screen for emerging technologies that might become relevant in the future. In total 179 patents were found, out of which 25 were evaluated by screening the title and abstract to be relevant to the field. [ABSTRACT FROM AUTHOR]

Published

2015

40. Human T-Cell Cloning by Limiting Dilution

Author

Manuela Capone, Alessio Mazzoni, and Laura Maggi

Subjects

0301 basic medicine, T cell, Cell, T-cell receptor, Biology, Phenotype, In vitro, Cell biology, T cell cloning, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, medicine.anatomical_structure, Limiting dilution, medicine, Function (biology), 030215 immunology

Abstract

Human T cells represent a heterogeneous population, including cells with different phenotypical and function properties. Despite, in the last years, several technologies were developed to investigate phenotypical properties of T cells at single cell level, in vitro T cell clone 's culture remains the only way to perform functional study on T cells at single cell levels. Here, we describe the method to obtain human T cell clones by limiting dilution in the presence of feeder cells and to maintain them in culture for further investigations.

Published

2021

41. Development and characterization of monoclonal antibodies against human IgA in Balb/c mice.

Author

Ezzatifar, Fatemeh, Majidi, Jafar, Baradaran, Behzad, Maleki, Leili Aghebati, Abdolalizadeh, Jalal, and Yousefi, Mehdi

Subjects

*IMMUNOGLOBULIN A, *MONOCLONAL antibodies, *DIAGNOSTIC equipment, *ENZYME-linked immunosorbent assay, *LABORATORY mice

Abstract

OBJECTIVE: Immunoglobulin A (IgA) is the second immunoglobulin in human serum. Monoclonal antibodies have many potential uses in diagnosis, treatment and purification. The conjugated monoclonal antibodies against human IgA are utilized in diagnostic kits. METHODS: For production of monoclonal antibodies against human Immunoglobulin A, spleen cells of the immune mouse were fused with SP2/0 as myeloma cells and Poly Ethylene Glycol (PEG). Supernatant of hybridoma cells was screened to determine the antibody by ELISA. The appropriate clones were selected for limiting dilution (L.D). Ultimately, appropriate monoclone was injected intraperitoneally into the mouse that has been primed with Pristane.RESULTS: In current study, 175 clones were obtained of which 5 clones had absorbance values of about 3 were selected for limiting dilution. Between these clones, 3-D5monoclone with IgG1 subclass was selected as appropriate one and it was reproduced in FCS free RPMI 1640. For large scale production in invivo, the appropriate clone was implanted in the peritoneum of the Balb/c mouse and its titer was determined, which showed 1/100,000 dilution for ascitic fluid, having no cross reactivity with IgM & IgG. CONCLUSIONS: Monoclonal antibody was purified by chromatography, confirmed by SDS-PAGE and then conjugated with enzyme and used for diagnostic kits. [ABSTRACT FROM AUTHOR]

Published

2014

42. Patient-Specific Minimal Residual Disease Primers Amplify with Uniformly High Efficiency

Author

Elizabeth Hughes, Sue Latham, Alexander A. Morley, Paul A. Bartley, and Bradley Budgen

Subjects

0301 basic medicine, Neoplasm, Residual, Population, Biology, Polymerase Chain Reaction, Sensitivity and Specificity, Pathology and Forensic Medicine, law.invention, 03 medical and health sciences, 0302 clinical medicine, law, Limiting dilution, Biomarkers, Tumor, Humans, education, Polymerase chain reaction, DNA Primers, education.field_of_study, Reproducibility of Results, Patient specific, Minimal residual disease, Molecular biology, 030104 developmental biology, 030220 oncology & carcinogenesis, Molecular Medicine, Primer (molecular biology), Immunoglobulin Heavy Chains

Abstract

The widespread use of PCR to quantify minimal residual disease has been hampered by the apparently wide variation in amplification efficiency (AE) of PCR primers. A new method to measure AE was developed on the basis of the Ct results of PCR amplification of single copies of a target molecule placed by limiting dilution into wells of a microplate. The mean one copy Ct of a population of primers or of a reference primer was calibrated against the AE determined by the standard method of regression analysis. The AE of a test primer could then be determined by relating its one copy Ct value to the calibrated mean one copy Ct value. This new method was much more precise than direct determination of AE by regression analysis. The AE of minimal residual disease primers, and of primers for eight other genes, was determined to be >95% and often close to 100%. A primer/plasmid standard was produced to enable transfer of the method to other laboratories. The one copy Ct method thus enables AE of a patient-specific primer to be simply and accurately determined.

Published

2020

43. Methods for Automated Single Cell Isolation and Sub‐Cloning of Human Pluripotent Stem Cells

Author

Narasimha Swamy Telugu, Sandra Schommer, Iris Fischer, Valeria Fernandez Vallone, Duncan C. Miller, Harald Stachelscheid, and Sebastian Diecke

Subjects

Pluripotent Stem Cells, 0301 basic medicine, Genetic stability, Cell Culture Techniques, Cell Separation, Computational biology, Biology, 03 medical and health sciences, 0302 clinical medicine, Genome editing, Limiting dilution, Humans, CRISPR, Cell isolation, Cloning, Molecular, Induced pluripotent stem cell, Protocol (object-oriented programming), Automation, Laboratory, Gene Editing, Cloning, Cell Biology, General Medicine, Clone Cells, 030104 developmental biology, Single-Cell Analysis, 030217 neurology & neurosurgery, Developmental Biology

Abstract

Advances in human pluripotent stem cell (hPSC) techniques have led them to become a widely used and powerful tool for a vast array of applications, including disease modeling, developmental studies, drug discovery and testing, and emerging cell-based therapies. hPSC workflows that require clonal expansion from single cells, such as CRISPR/Cas9-mediated genome editing, face major challenges in terms of efficiency, cost, and precision. Classical sub-cloning approaches depend on limiting dilution and manual colony picking, which are both time-consuming and labor-intensive, and lack a real proof of clonality. Here we describe the application of three different automated cell isolation and dispensing devices that can enhance the single-cell cloning process for hPSCs. In combination with optimized cell culture conditions, these devices offer an attractive alternative compared to manual methods. We explore various aspects of each device system and define protocols for their practical application. Following the workflow described here, single cell-derived hPSC sub-clones from each system maintain pluripotency and genetic stability. Furthermore, the workflows can be applied to uncover karyotypic mosaicism prevalent in bulk hPSC cultures. Our robust automated workflow facilitates high-throughput hPSC clonal selection and expansion, urgently needed in the operational pipelines of hPSC applications. © 2020 The Authors. Basic Protocol: Efficient automated hPSC single cell seeding and clonal expansion using the iotaSciences IsoCell platform Alternate Protocol 1: hPSC single cell seeding and clonal expansion using the Cellenion CellenONE single-cell dispenser Alternate Protocol 2: hPSC single cell seeding and clonal expansion using the Cytena single-cell dispenser Support Protocol 1: Coating cell culture plates with Geltrex Support Protocol 2: hPSC maintenance in defined feeder-free conditions Support Protocol 3: hPSC passaging in clumps Support Protocol 4: Laminin 521 coating of IsoCell plates and 96-well/384-well plates Support Protocol 5: Preparation of medium containing anti-apoptotic small molecules Support Protocol 6: 96- and 384-well target plate preparation prior to single cell seeding Support Protocol 7: Single cell dissociation of hPSCs Support Protocol 8: IsoCell-, CellenONE-, and Cytena-derived hPSC clone subculture and expansion.

Published

2020

44. Inter-Laboratory Reproducibility of Inducible HIV-1 Reservoir Quantification by TILDA

Author

Cynthia Lungu, Jolanda J.C. Voermans, Shringar Rao, Casper Rokx, Francesco A. Procopio, Jeroen J. A. van Kampen, Rob J J Beerkens, Tokameh Mahmoudi, David A. M. C. van de Vijver, Ronald J Overmars, Giuseppe Pantaleo, Rob A. Gruters, Charles A. Boucher, Henrieke A. B. Prins, Virology, Biochemistry, Medical Microbiology & Infectious Diseases, and Internal Medicine

Subjects

Adult, CD4-Positive T-Lymphocytes, Male, 0301 basic medicine, Computer science, 030106 microbiology, Human immunodeficiency virus (HIV), lcsh:QR1-502, HIV Infections, Computational biology, medicine.disease_cause, Hiv 1 latency, lcsh:Microbiology, Young Adult, 03 medical and health sciences, inducible reservoirs, Proviruses, SDG 3 - Good Health and Well-being, Virology, Limiting dilution, medicine, Humans, Inter-laboratory, reservoir quantification, Reproducibility, Brief Report, Reproducibility of Results, Robustness (evolution), Middle Aged, Provirus, Virus Latency, 3. Good health, 030104 developmental biology, Infectious Diseases, Concordance correlation coefficient, assay performance, HIV-1, Female, HIV-1 latency, TILDA, Laboratories

Abstract

Substantial efforts to eliminate or reduce latent HIV-1 reservoirs are underway in clinical trials and have created a critical demand for sensitive, accurate, and reproducible tools to evaluate the efficacy of these strategies. Alternative reservoir quantification assays have been developed to circumvent limitations of the quantitative viral outgrowth assay. One such assay is tat/rev induced limiting dilution assay (TILDA), which measures the frequency of CD4+ T cells harboring inducible latent HIV-1 provirus. We modified pre-amplification reagents and conditions (TILDA v2.0) to improve assay execution and first internally validated assay performance using CD4+ T cells obtained from cART-suppressed HIV-1-infected individuals. Detection of tat/rev multiply spliced RNA was not altered by modifying pre-amplification conditions, confirming the robustness of the assay, and supporting the technique’s amenability to limited modifications to ensure better implementation for routine use in clinical studies of latent HIV-1 reservoirs. Furthermore, we cross-validated results of TILDA v2.0 and the original assay performed in two separate laboratories using samples from 15 HIV-1-infected individuals. TILDA and TILDA v2.0 showed a strong correlation (Lin’s Concordance Correlation Coefficient = 0.86). The low inter-laboratory variability between TILDAs performed at different institutes further supports use of TILDA for reservoir quantitation in multi-center interventional HIV-1 Cure trials.

Published

2020

45. Measuring the Inducible, Replication-Competent HIV Reservoir Using an Ultra-Sensitive p24 Readout, the Digital ELISA Viral Outgrowth Assay

Author

Erin L. Stuelke, Katherine S. James, Jennifer L. Kirchherr, Brigitte Allard, Caroline Baker, Joann D. Kuruc, Cindy L. Gay, David M. Margolis, and Nancie M. Archin

Subjects

CD4-Positive T-Lymphocytes, lcsh:Immunologic diseases. Allergy, 0301 basic medicine, Cell, Immunology, IUPM, HIV Core Protein p24, Human immunodeficiency virus (HIV), Enzyme-Linked Immunosorbent Assay, HIV Infections, Stimulation, Biology, Virus Replication, medicine.disease_cause, Sensitivity and Specificity, Peripheral blood mononuclear cell, Virus, 03 medical and health sciences, 0302 clinical medicine, Limiting dilution, medicine, Humans, Immunology and Allergy, Latency (engineering), Ultra sensitive, Original Research, HIV, Viral Load, Virology, 030104 developmental biology, medicine.anatomical_structure, DEVO, outgrowth, HIV-1, QVOA, lcsh:RC581-607, 030215 immunology

Abstract

Quantifying the inducible HIV reservoir provides an estimate of the frequency of quiescent HIV-infected cells in humans as well as in animal models, and can help ascertain the efficacy of latency reversing agents (LRAs). The quantitative viral outgrowth assay (QVOA) is used to measure inducible, replication competent HIV and generate estimations of reservoir size. However, traditional QVOA is time and labor intensive and requires large amounts of lymphocytes. Given the importance of reproducible and accurate assessment of both reservoir size and LRA activity in cure strategies, efforts to streamline the QVOA are of high priority. We developed a modified QVOA, the Digital ELISA Viral Outgrowth or DEVO assay, with ultra-sensitive p24 readout, capable of femtogram detection of HIV p24 protein in contrast to the picogram limitations of traditional ELISA. For each DEVO assay, 8–12 × 106 resting CD4 + T cells from aviremic, ART-treated HIV + participants are plated in limiting dilution and maximally stimulated with PHA, IL-2 and uninfected allogeneic irradiated PBMC. CD8-depleted PHA blasts from an uninfected donor or HIV-permissive cells (e.g., Molt4/CCR5) are added to the cultures and virus allowed to amplify for 8–12 days. HIV p24 from culture supernatant is measured at day 8 by Simoa (single molecule array, ultra-sensitive p24 assay) confirmed at day 12, and infectious units per million CD4 + T cells (IUPM) are calculated using the maximum likelihood method. In all DEVO assays performed, HIV p24 was detected in the supernatant of cultures as early as 8 days post stimulation. Importantly, DEVO IUPM values at day 8 were comparable or higher than traditional QVOA IUPM values obtained at day 15. Interestingly, DEVO IUPM values were similar with or without the addition of allogeneic CD8-depleted target PHA blasts or HIV permissive cells traditionally used to expand virus. The DEVO assay uses fewer resting CD4 + T cells and provides an assessment of reservoir size in less time than standard QVOA. This assay offers a new platform to quantify replication competent HIV during limited cell availability. Other potential applications include evaluating LRA activity, and measuring clearance of infected cells during latency clearance assays.

Published

2020

46. Current status and detection of genetically modified organism

Author

TZU-MING PAN

Subjects

Pharmacology, 0303 health sciences, food.ingredient, Genetically modified maize, 030309 nutrition & dietetics, business.industry, fungi, 010401 analytical chemistry, food and beverages, Herbicide tolerant crops, Genetically modified crops, 01 natural sciences, 0104 chemical sciences, Biotechnology, Genetically modified organism, 03 medical and health sciences, Geography, food, Limiting dilution, business, Canola, Food Science

Abstract

Production of genetically modified (GM) crops is currently concentrated in just a few countries. In 2001, 99% of GM crops was produced in four countries: US 68%, Argentina 11.8%, Canada 6% and China 3%. Crop-wise, GM soybean made up 63% of global GM planting area and GM corn accounts for 19%, followed by GM cotton (13%) and GM canola (5%). In terms of the global planting ar ea, GM soybean and cotton accounted for 46% and 20%, respectively. Two major genetically modified organisms (GMO) traits in 2001 were herbicide tolerant crops, accounted for 77% of all GM crops, while Bt maize accounted for 11%. Legislation enacted worldwide to regulate the presence of GMOs in crops, foods and ingredients, necessitated the development of reliable and sensitive methods for GMO detection. In this article, protein- and DNA-based methods employing western blots, enz ymelinked immunosorbant assay, lateral flow strips, Southern blots, qualitative-, quantitative-, real-time- and limiting dilution- PCR methods, are discussed. Where information on modified gene sequences is not available, new approaches, such as near-infrared spectromet ry, might tackle the problem of detection of non-approved genetically modified (GM) foods. The efficiency of screening, identifica tion and confirmation strategies should be examined with respect to false-positive rates, disappearance of marker genes, increased use o f specific regulator sequences and the increasing number of GM foods.

Published

2020

47. Differences in inducibility of the latent HIV reservoir in perinatal and adult infection

Author

Adit Dhummakupt, Thuy Anderson, Allison L. Agwu, Jessica H. Rubens, Bareng A. S. Nonyane, Lilly V. Siems, R. Brad Jones, Deborah Persaud, Laura Powell, Tricia L. Nilles, Vicki Tepper, and Aleisha Collinson-Streng

Subjects

Adult, CD4-Positive T-Lymphocytes, 0301 basic medicine, Adolescent, T cell, Human immunodeficiency virus (HIV), HIV Infections, Stimulation, Virus Replication, medicine.disease_cause, Antiviral Agents, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Pregnancy, Limiting dilution, Humans, Medicine, Latency (engineering), Disease Reservoirs, business.industry, General Medicine, Viral Load, Virus Latency, 030104 developmental biology, medicine.anatomical_structure, chemistry, 030220 oncology & carcinogenesis, Ionomycin, Immunology, HIV-1, Female, business, Immunologic Memory, Ex vivo, Research Article, Immune activation

Abstract

The HIV latent reservoir in resting memory CD4(+) T cells precludes cure. Therapeutics to reactivate and eliminate this reservoir are in clinical trials in adults, but not yet in pediatric populations. We determined, ex vivo, the inducibility of the latent reservoir in perinatal infection as compared with adult infections using the Tat/rev induced limiting dilution assay (TILDA), in which a single round (12 hours) of CD4(+) T cell stimulation with PMA/ionomycin maximally activates T cells and leads to proviral expression with multiply spliced HIV RNA production. Markers of immune activation and exhaustion were measured to assess interactions with inducibility. Although rates of T cell activation with PMA/ionomycin were similar, the latent reservoir in perinatal infection was slower to reactivate and of lower magnitude compared with adult infection, independent of proviral load. An enhanced TILDA with the addition of phytohemagglutin and a duration of 18 hours augmented proviral expression in perinatal but not adult infection. The baseline HLA-DR(+)CD4(+) T cell level was significantly lower in perinatal compared with adult infections, but not correlated with induced reservoir size. These data support the hypothesis that there are differences in kinetics of latency reversal and baseline immune activation in perinatal compared with adult infections, with implications for latency reversal strategies toward reservoir clearance and remission.

Published

2020

48. Optimized Protocol for Testing Multipurpose Contact Lens Solution Efficacy Against Acanthamoeba

Author

Jeffrey M Brocious, Katherine D Adams, Denise Hampton, Malvina B. Eydelman, Daniel P Fedorko, and Victoria M. Hitchins

Subjects

0301 basic medicine, Positive control, Acanthamoeba, Neutralization, Microbiology, 03 medical and health sciences, 0302 clinical medicine, Most probable number, Limiting dilution, parasitic diseases, Humans, Amebicides, Trophozoites, Acanthamoeba castellanii, biology, Cysts, Chemistry, Reproducibility of Results, Hydrogen Peroxide, biology.organism_classification, Contact lens, Ophthalmology, 030104 developmental biology, Acanthamoeba polyphaga, Acanthamoeba Keratitis, 030221 ophthalmology & optometry, Contact Lens Solutions, Disinfectants

Abstract

OBJECTIVES To evaluate the interlaboratory and intralaboratory reproducibility of a proposed protocol for multipurpose contact lens solution (MPS) disinfection efficacy against Acanthamoeba. METHODS Acanthamoeba castellanii and Acanthamoeba polyphaga and four MPS with different biocidal agents were used to evaluate the protocol in two different laboratories. In addition to the negative control, a positive control and neutralization control were used. One experiment was performed in triplicate, and all other experiments were performed in duplicate in each laboratory. Acanthamoeba trophozoites were grown axenically, and cysts were generated using the starvation method. Trophozoites and cysts at a concentration of 2.0 × 10 to 2.0 × 10 organisms per milliliter were exposed to the test MPS for 0, 4 or 6 (manufacturer's recommended soak time [MRST]), 8, and 24 hr. Survivors were determined by a limiting dilution method that used a most probable number evaluation. RESULTS The positive and negative controls displayed consistent results and trends both within each laboratory and between each laboratory for trophozoites and cysts of both A. castellanii and A. polyphaga. The neutralization control consistently demonstrated the ability of the neutralizing agents to neutralize the MPS and the positive control and demonstrated no inhibition of Acanthamoeba by the negative control. Testing in triplicate and duplicate demonstrated the reproducibility of the protocol both within each laboratory and between the laboratories. Our results demonstrated that the MPS at the MRST and at 8 hr (likely overnight soak time) are generally more effective against trophozoites than they are against cysts. Only the MPS with hydrogen peroxide as the biocidal agent was able to provide a greater than three-log kill of cysts at the MRST and longer. Among the MPS we tested, trophozoites of A. castellanii and A. polyphaga showed similar responses. Some variability was observed when testing cysts of both species. In both laboratories, one nonhydrogen peroxide containing MPS had some effect (>1 log kill) on A. polyphaga cysts. This solution had no effect (

Published

2018

49. Impact of pre-amplification conditions on sensitivity of the tat/rev induced limiting dilution assay

Author

Xuefen Yang, Hugo Soudeyns, Paul Sandstrom, Liam Châtel, François Cholette, and Carole Lavigne

Subjects

CD4-Positive T-Lymphocytes, 0301 basic medicine, medicine.medical_specialty, HIV Infections, Viremia, Biology, Polymerase Chain Reaction, Sensitivity and Specificity, Cell Line, law.invention, 03 medical and health sciences, Medical microbiology, law, Virology, Limiting dilution, medicine, Humans, Polymerase chain reaction, Measurement method, Macrophages, RNA, rev Gene Products, Human Immunodeficiency Virus, General Medicine, Gold standard (test), Viral Load, medicine.disease, Antiretroviral therapy, Virus Latency, 3. Good health, 030104 developmental biology, Anti-Retroviral Agents, HIV-1, RNA, Viral, tat Gene Products, Human Immunodeficiency Virus

Abstract

Antiretroviral therapy (ART) can lower a patient’s HIV plasma viral load to an undetectable level, but following cessation of ART viremia rapidly rebounds. It has been shown that ART does not eliminate latent viruses sequestered into anatomical and cellular reservoirs. Therefore, in patients that have ceased ART, the following rebound in HIV viremia is caused by the activation of latent HIV reservoirs. A major issue in HIV cure research is the quantification of these latent HIV reservoirs. Various reservoir measurement methods exist, but the gold standard technique remains the culture-based quantitative viral outgrowth assay (QVOA). Recently, a new PCR-based assay, named the tat/rev induced limiting dilution assay (TILDA) was described which measures the frequency of inducible latently infected CD4+ T cells that actively produce multiply-spliced RNA coding for the Tat/Rev proteins. The objective of this study was to further optimize the assay by examining the influence of varied factors, such as the amount of products transferred from the pre-amplification step to the PCR reaction, storage of pre-amplification products prior to PCR runs, and the number of cells used, on the assay’s sensitivity and reproducibility. We also investigated whether the assay could be used to quantify HIV reservoirs in monocytes/macrophages.

Published

2018

50. Functional assessment of spermatogonial stem cell purity in experimental cell populations

Author

Jon M. Oatley and Tessa Lord

Subjects

0301 basic medicine, Male, Cell, Population, Computational biology, Biology, Article, 03 medical and health sciences, Mice, Limiting dilution, medicine, Animals, education, lcsh:QH301-705.5, Progenitor, education.field_of_study, Transplantation, Stem Cells, Cell Biology, General Medicine, Spermatogonia, 030104 developmental biology, medicine.anatomical_structure, lcsh:Biology (General), Colony count, Stem cell, Spermatogonial stem cell, Stem cell biology, Developmental Biology, Stem Cell Transplantation

Abstract

Historically, research in spermatogonial biology has been hindered by a lack of validated approaches to identify and isolate pure populations of the various spermatogonial subsets for in-depth analysis. In particular, although a number of markers of the undifferentiated spermatogonial population have now been characterized, standardized methodology for assessing their specificity to the spermatogonial stem cell (SSC) and transit amplifying progenitor pools has been lacking. To date, SSC content within an undefined population of spermatogonia has been inferred using either lineage tracing or spermatogonial transplantation analyses which generate qualitative and quantitative data, respectively. Therefore, these techniques are not directly comparable, and are subject to variable interpretations as to a readout that is representative of a ‘pure’ SSC population. We propose standardization across the field for determining the SSC purity of a population via use of a limiting dilution transplantation assay that would eliminate subjectivity and help to minimize the generation of inconsistent data on ‘SSC’ populations. In the limiting dilution transplantation assay, a population of LacZ-expressing spermatogonia are selected based on a putative SSC marker, and a small, defined number of cells (i.e. 10 cells) are microinjected into the testis of a germ cell-deficient recipient mouse. Using colony counts and an estimated colonization efficiency of 5%; a quantitative value can be calculated that represents SSC purity in the starting population. The utilization of this technique would not only be useful to link functional relevance to novel markers that will be identified in the future, but also for providing validation of purity for marker-selected populations of spermatogonia that are commonly considered to be SSCs by many researchers in the field of spermatogenesis and stem cell biology. Keywords: Spermatogonial stem cell, Limiting dilution, Transplantation

Published

2018