Considerations of Cell Counting Analysis when using Different Types of Cells
Beckman Coulter Life Sciences is proud to introduce our new Vi-CELL BLU Cell Viability Analyzer. The Vi-CELL BLU leverages the key performance features of the Vi-CELL XR but incorporates many design improvements that our customers have requested over the years.
While a seemingly straightforward application, automated cell counting can be influenced by a variety of conditions and variables arising from both the sample and instrument. With the new Vi-CELL BLU we have introduced the capability to load 96 samples into a standard plate and run this as a single experiment. However this requires approximately 3 hours to run the entire plate with may not be ideal, particularly for cell types that generally have low viability or are prone deterioration once outside the incubator or bioreactor.
The plate loader also allows us to assess multiple different experimental conditions in a single run thus providing the opportunity to evaluate a range of conditions or criteria.
To demonstrate these capabilities we reviewed several different cell types and cell preparation approaches using standard cells.
Cell Counting Analysis
Cells cultures of CHO (Chinese Hamster Ovary), EL4 (Mouse T Lymphocyte Cell Line), SF9 (Ovarian tissue from Spodoptera frugiperda) insect cells and of HELA cells were used to assess the effects of long analysis durations and different sample preparation conditions on different types of cells.
CHO Cell Sample Preparation Impact
Centrifugation and resuspension are routine methods for washing and concentrating cells ahead of reseeding or use in other experiments. CHO cells are generally considered to quite durable, but they do have very particular growth requirements and require specialized media for best health. In the experiment below the cells were centrifuged at 1000 g for 5 minutes, a relatively mild spin before being resuspended in media or buffer to assess the impact, if any, of cell preparation on cell health
Results
| Treatment | Concentration (M/mL) | Viability (%) | Diameter (µm) |
| Untreated | 4.83 | 94.30 | 16.12 |
| 1 spin resuspend in media | 5.05 | 94.48 | 16.17 |
| 1 spin resuspend in PBS | 4.70 | 65.69 | 14.17 |
| 2 spins resuspend in PBS | 4.45 | 53.77 | 13.99 |
The results show that centrifugation and resuspension in recommended media has no appreciable impact on the CHO cells. However resuspension in PBS buffer results in a drastic loss of viability and significant reduction in average cell diameter. There is also some minor reduction in cell concentration which may be expected from losses during resuspension. Spinning and resuspending a second time in PBS has a further negative impact on cell viability and cell size
Figure 2. Impact of sample preparation method on CHO cells
EL4 Cells Mixing Cycle Analysis
EL4 cells are generally considered to be fragile and even under ideal conditions grow slowly and show viability <70%. EL4 cells were prepared and dispensed into a 96 well plate. Cell Type profiles were created using the standard Mammalian cell profile as source and differing levels of mixing cycles. The goal was to assess the impact, if any, of increased agitation on a cell type known to be easily damaged by vortex mixing and centrifugation
Results
The results for the EL4 cells are given below:
| Mix Cycles | Cell Count | Viable Cell Count | Concentration (M/mL) | Viability (%) | Diameter (µm) |
| 1 | 4648 | 2837 | 1.72 | 61.06 | 11.34 |
| 3 | 4637 | 2715 | 1.72 | 58.54 | 11.34 |
| 5 | 4660 | 2582 | 1.73 | 55.69 | 11.34 |
| 7 | 4660 | 2448 | 1.73 | 52.53 | 11.32 |
While the cell counts, concentration and diameter values show no statistical significance there is a marked drop in viable cell count and consequently in cell viability with increased mixing cycles across all dilutions. This may indicate that a Cell Type Profile with reduced aspiration and mixing cycles may be more suitable for this type of cell and excessive agitation may not be ideal and should be avoided
Figure 3. Impact of mixing cycles on EL4 cells
SF9 Insect Cells
Even when grown under ideal conditions SF9 cells do not achieve high densities easily and typically have viability below 60%. It is therefore possible that the prolonged instrument time required for a plate run may negatively impact the cell culture. To assess this SF9 cells were plated and run using the standard Insect Cell profile.
The results show that over the course of the 3 hour run there was no detectable impact on cell viability and no notable change in cell diameter that may occur if the cells are dying or swelling. As such it would appear this cell line, although low in viability, is robust enough to spend extended periods outside the cell incubator environment without adverse effects
Figure 4. Viability and average diameter of SF9 cells over time. No significant change noted over course of experiment.
HELA Cell Cultures
HELA cells were grown to a high state of confluence in order to stress the cells. The cells were then harvested and dispersed into suspension. The cells were then plated out on a 96 well plate and data collected using standard Mammalian cell profile. The plate was run collecting data by columns to ensure the same time interval between samples in the rows.
It was noted that the later samples in the plate run were reporting slightly higher concentrations. Further investigations showed that the cells were increasing in average diameter as time progressed.
Figure 5. Percentage increase in average diameter of HELA cells over time
Viewing the acquired images shows an increasing number of cells which appear to be swelling or blebbing along with a large number of non-cellular vesicles. While the latter do not usually impact the cell count, depending on the cell profile settings, they could be counted as small cells. The swelling effect causes the average cell diameter to increase almost 10% over the course of the 3 hours it takes to run the plate and may cause some smaller cells just below the lower diameter threshold to become included in the cell counts.
Figure 6. Cell swelling and blebbing in HELA cells after >2hrs outside incubator
Conclusions
It is recommended that prior to running a cell culture on a complete plate that some initial evaluation is performed to determine the robustness of the cells involved and their ability to tolerate the sample preparation methods and prolonged exposure outside the incubator environment. Even engineered cells such as CHO cells or immortal HELA cells, which are generally selected to be quite durable, can be effect by stress or particular sample preparation conditions.
Helpful Links
-
Material de Leitura
-
Notas de Aplicação
- 17-Marker, 18-Color Human Blood Phenotyping Made Easy with Flow Cytometry
- 21 CFR Part 11 Data Integrity for On-line WFI Instruments
- 8011+ Reporting Standards Feature and Synopsis
- Achieving Compliant Batch Release – Sterile Parenteral Quality Control
- Air Particle Monitoring ISO 21501-4 Impact
- An Analytical Revolution: Introducing the Next Generation Optima AUC
- Analyzing Mussel/Mollusk Propagation using the Multisizer 4e Coulter Counter
- Automated 3D Cell Culture and Screening by Imaging and Flow Cytometry
- Automated Cell Plating and Growth Assays
- Automated Cell Transfection and Reporter Gene Assay
- Automated Cord Blood Cell Viability and Concentration Measurements Using the Vi‑CELL XR
- Automated Genomic Sample Prep-Ampure XP PCR
- Automated Genomic Sample Prep-RNAdvance
- Automated Genomic Sample Prep-Sample Quality Control
- Automated salt-assisted liquid-liquid extraction
- Automated Sample Preparation for the Monitoring of Pharmaceutical and Illicit Drugs by LC-MS/MS
- Automated Transfection Methods
- Automated XTT Assay for Cell Viability Analysis
- Automating a Linear Density Gradient for Purification of a Protein:Ligand Complex
- Automating Biopharma Quality Control to Reduce Costs and Improve Data Integrity
- Automating Bradford Assays
- Automating Cell Line Development
- Automating Cell Line Development
- Automating Cell-Based Processes
- Automating the Cell Line Development Workflow
- The new Avanti J-15 Centrifuge Improves Sample Protection and Maximizes Sample Recovery
- The New Avanti J-15 Centrifuge Time Saving Deceleration Profile Improves Workflow Efficiency
- Avanti JXN Protein Purification Workflow
- Avoid the Pitfalls When Automating Cell Viability Counting for Biopharmaceutical Quality Control
- Beer, Evaluation of Final Product and Filtration Efficiency
- Biomek Automated Genomic Sample Prep Accelerates Research
- Biomek Automated NGS Solutions Accelerate Genomic Research
- Preparation and purification of carbon nanotubes using an ultracentrifuge and automatic dispensing apparatus, and analysis using an analytical centrifuge system
- Cell Counting Performance of Vi–Cell BLU Cell Viability Analyzer
- Cell Line Development – Data Handling
- Cell Line Development – Hit Picking
- Cell Line Development – Limiting Dilution
- Cell Line Development – Selection and Enrichment
- Changes to GMP Force Cleanroom Re-Classifications
- Characterizing Insulin as a Biopharmaceutical Using Analytical Ultracentrifugation
- Clean Cabinet Air Particle Evaluation
- Cleanroom Routine Environmental Monitoring – FDA Guidance on 21 CFR Part 11 Data Integrity
- Comparing Data Quality & Optical Resolution of the Next Generation Optima AUC to the Proven ProteomeLab on a Model Protein System
- Conducting the ISO 14644-3 Cleanroom Recovery Test with the MET ONE 3400
- Considerations of Cell Counting Analysis when using Different Types of Cells
- Consistent Cell Maintenance and Plating through Automation
- Control Standards and Method Recommendations for the LS 13 320 XR
- Counting Efficiency: MET ONE Air Particle Counters and Compliance to ISO-21501
- Critical Particle Size Distribution for Cement using Laser Diffraction
- CytoFLEX
- Detecting Moisture in Hydraulic Fluid, Oil and Fuels
- Determination of Size and Concentration of Particles in Oils
- Efficient kit-free nucleic acid isolation uses a combination of precipitation and centrifugation separation methods
- dsDNA Quantification with the Echo 525 Liquid Handler for Miniaturized Reaction Volumes, Reduced Sample Input, and Cost Savings
- Compensation Setup For High Content DURAClone Reagents
- Echo System-Enhanced SMART-Seq v2 for RNA Sequencing
- Efficient Factorial Optimization of Transfection Conditions
- Enhancing Vaccine Development and Production
- Enumeration And Size Distribution Of Yeast Cells In The Brewing Industry
- European Pharmacopoeia EP 2.2.44 and Total Organic Carbon
- Evaluation of Instrument to Instrument Performance of the Vi-CELL BLU Cell Viability Analyzer
- Exosome-Depleted FBS Using Beckman Coulter Centrifugation: The cost-effective, Consistent choice
- Flexible ELISA automation with the Biomek i5 Workstation
- Full Automation of the SISCAPA® Workflow using a Biomek NXP Laboratory Automation Workstation
- Fully-Automated Cellular Analysis by Flow Cytometry
- Get Control in GMP Environments
- g-Max: Added Capabilities to Beckman Coulter's versatile Ultracentrifuge Line
- Grading of nanocellulose using a centrifuge
- A method of grading nanoparticles using ultracentrifugation in order to determine the accurate particle diameter
- Grading of pigment ink and measurement of particle diameter using ultracentrifugation / dynamic light scattering
- HIAC Industrial – Our overview solution for fluid power testing for all applications
- HIAC PODS+ Online Mode & Filter Cart Mode
- HIAC PODS+ versus Parker ACM-20 Performance comparison
- A complete workflow for high-throughput isolation of DNA and RNA from FFPE samples using Formapure XL Total on the KingFisher™ Sample Purification System: an application for robust and scalable cancer research and biomarker discovery
- A Highly Consistent BCA Assay on Biomek i-Series
- A Highly Consistent Bradford Assay on Biomek i-Series
- A Highly Consistent Lowry Method on Biomek i-Series
- Highly Reproducible Automated Proteomics Sample Preparation on Biomek i-Series
- Cell Line Development – Hit Picking
- Como Usar o Side Scatter do laser Violeta para Detectar Nanopartículas no Citômetro de Fluxo CytoFLEX
- How Violet Side Scatter Enables Nanoparticle Detection
- HRLD Recommended Volume Setting
- Hydraulic Oil Measurement
- ICH Q2 – the Challenge of Measuring Total Organic Carbon in Modern Pharmaceutical Water Systems
- ICH Q2 – The Challenge of Measuring Total Organic Carbon in Modern Pharmaceutical Water Systems
- Importance of TOC measurement in WFI in light of European Pharmacopoeia change
- Temperature dependence of hydrodynamic radius of an intrinsically disordered protein measured in the Optima AUC analytical ultracentrifuge.
- Isolation of cell-free DNA (cfDNA) from plasma using Apostle MiniMax™ High Efficiency cfDNA Isolation kit— comparison of fully automated, semi-automated and manual workflow processing
- Issues with Testing Jet Fuels for Contamination
- Leveraging the Vi-CELL MetaFLEX for Monitoring Cell Metabolic Activity
- Linearity of BSA Using Absorbance & Interference Optics
- Long Life Lasers
- LS 13 320 XR: Sample Preparation - How to measure success
- Particle Size Analysis Simple, Effective and Precise
- Matching Cell Counts between Vi–CELL XR and Vi–CELL BLU
- MET ONE Sensor Verification
- Metal colloid purification and concentration using ultracentrifugation
- Separation and purification of metal nanorods using density gradient centrifugation
- Method for Determining Cell Type Parameter Adjustment to Match Legacy Vi CELL XR
- Minimal Sample to Sample Carry Over with the HIAC 8011+
- Minimizing process variability in the manufacturing of bottled drinking water
- Modern Trends in Non‐Viable Particle Monitoring during Aseptic Processing
- Multi-Wavelength Analytical Ultracentrifugation of Human Serum Albumin complexed with Porphyrin
- Particle diameter measurement of a nanoparticle composite - Using density gradient ultracentrifugation and dynamic light scattering
- What to do now that ACFTD is discontinued
- Optimizing the HIAC 8011+ Particle Counter for Analyzing Viscous Fluids
- Optimizing the Multisizer 4e Coutler Counter for use with Small Apertures
- Optimizing Workflow Efficiency of Cleanroom Routine Environmental Monitoring
- Particle Counting in Mining Applications
- Particle testing in cleanroom high-pressure gas lines to ISO 14644 made easy with the MET ONE 3400 gas calibrations
- Pharma Manufacturing Environmental Monitoring
- Pharma Manufacturing Paperless Monitoring
- Principles of Continuous Flow Centrifugation
- Protein purification workflow
- Background Subtraction
- Calibrating the QbD1200 TOC Analyzer
- Detection Limit
- Inorganic Carbon Removal
- JP SDBS Validation
- Method Overview
- Overload Recovery
- QbD1200 Preparing Reagent Solution
- USP System Suitability
- Quality Control Electronic Records for 21 CFR part 11 Compliance
- Using the Coulter Principle to Quantify Particles in an Electrolytic Solution for Copper Acid Plating
- RCC A standardized automated approach for exosome isolation and characterization
- RCC Avanti J 15 Series Maximizing Sample Protection and Sample Recovery
- RCC Avanti J 15 Series Time Savings and Workflow Efficiency
- Root Cause Investigations for Pharmaceutical Water Systems
- Scalable Plasmid Purification using CosMCPrep
- Specification Comparison of Vi–CELL XR and Vi–CELL BLU
- Specifying Non-Viable Particle Monitoring for Aseptic Processing
- A Standardized, Automated Approach For Exosome Isolation And Characterization Using Beckman Coulter Instrumentation
- Switching from Oil Testing to Water and back using the HIAC 8011+ and HIAC PODS+
- Advanced analysis of human T cell subsets on the CytoFLEX flow cytometer using a 13 color tube-based DURAClone dry reagent
- Using k-Factor to Compare Rotor Efficiency
- USP 787 Small Volume Testing
- Validation of On-line Total Organic Carbon Analysers for Release Testing Using ICH Q2
- Vaporized Hydrogen Peroxide Decontamination of Vi–CELL BLU Instrument
- Vi CELL BLU FAST Mode Option
- Vi-CELL BLU Regulatory Compliance - 21 CFR Part 11
- A workflow for medium-throughput isolation of cfDNA from plasma samples using Apostle MiniMax™ on the KingFisher™ Technology
- Using Machine Learning Algorithms to Provide Deep Insights into Cellular Subset Composition
- MET ONE 3400
- Miniaturization and Rapid Processing of TXTL Reactions Using Acoustic Liquid Handling
- Miniaturized Multi-Piece DNA Assembly Using the Echo 525 Liquid Handler
- Brochures, Flyers and Data Sheets
- Catalogs
- Flyers
-
Posters
- Applications of Ultracentrifugation in Purification and Characterization of Biomolecules
- Automating Genomic DNA Extraction from Whole Blood and Serum with GenFind V3 on the Biomek i7 Hybrid Genomic Workstation
- ABRF 2019: Automated Genomic DNA Extraction from Large Volume Whole Blood
- AACR 2019: Isolation and Separation of DNA and RNA from a Single Tissue or Cell Culture Sample
- AACR 2019: Correlation between Mutations Found in FFPE Tumor Tissue and Paired cfDNA Samples
- AGBT 2019: A Scalable and Automatable Method for the Extraction of cfDNA
- ABRF 2019: Simultaneous DNA and RNA Extraction from Formalin-Fixed Paraffin Embedded (FFPE) Tissue
- AMP 2019: Correlation Between Mutations Found in FFPE Tumor Tissue and Paired cfDNA Samples
- Automated library preparation for the MCI Advantage Cancer Panel at Miami Cancer Institute utilizing the Beckman Coulter Biomek i5 Span-8 NGS Workstation
- Automating Cell Line Development for Biologics
- Cellular Challenges: Taking an Aim at Cancer
- Cell-Line Engineering
- Characterizing the Light-Scatter Sensitivity of the CytoFLEX Flow Cytometer
- ASHG 2019: Comparison between Mutation Profiles of Paired Whole Blood and cfDNA Samples
- ASHG 2019: Correlation Between Mutations Found in FFPE Tumor Tissue and Paired cfDNA Samples
- Mastering Cell Counting
- Preparing a CytoFLEX for Nanoscale Flow Cytometry
- A Prototype CytoFLEX for High-Sensitivity, Multiparametric Nanoparticle Analysis
- Product Instructions
- Protocols
-
Case Studies
- Adenoviral Vectors Preparation
- Algae Biofuel Production
- Autophagy
- B Cell Research
- Basic Research on Reproductive Biology
- Cardiovascular Disease Research
- Cell Marker Analysis
- Choosing a Tabletop Centrifuge
- Collagen Disease Treatment
- Controlling Immune Response
- Creating Therapeutic Agents
- DNA Extraction from FFPE Tissue
- English Safety Seminar
- Equipment Management
- Exosome Purification Separation
- Future of Fishing Immune Research
- Hematopoietic Tumor Cells
- iPS Cell Research
- Membrane Protein Purification X Ray Crystallography
- Organelles Simple Fractionation
- Particle Interaction
- Retinal Cell Regeneration
- Sedimentary Geology
- Severe Liver Disease Treatment
- Treating Cirrhosis
- University Equipment Management
- Fundamentals of Ultracentrifugal Virus Purification
-
Whitepapers
- Centrifugation is a complete workflow solution for protein purification and protein aggregation quantification
- AUC Insights - Analysis of Protein-Protein-Interactions by Analytical Ultracentrifugation
- AUC Insights - Assessing the quality of adeno-associated virus gene therapy vectors by sedimentation velocity analysis
- AUC Insights - Sample concentration in the Analytical Ultracentrifuge AUC and the relevance of AUC data for the mass of complexes, aggregation content and association constants
- Hydraulic Particle Counter Sample Preparation
- eBooks
- Interviews
-
Notas de Aplicação