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Panel Design

 

Overview
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Multicolor flow cytometry is a powerful technology that enables simultaneous analysis of multiple markers at the single-cell level. With the increase in number of detectable parameters, the design of a multicolor panel can be challenging and requires an understanding of several factors that can influence panel performance:

 

  • Biology—Antigen density and co-expression
  • Fluorochrome—Brightness and spillover
  • Instrument—Configuration and set-up 
  • Explore pre-designed panels at the Interactive Cell Map

 

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Step 1

Define your experimental hypothesis

Defining your experimental hypothesis is the first step in panel design. Start with identifying:

  • The biological information you are trying to achieve
  • The population(s) of cells you wish to interrogate
  • Whether targets are found on the cell surface or intracellularly 
 
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Step 2

Marker selection

During the second step of the panel design process, you will need to identify which and how many markers you need to identify the population of interest.

Pay attention to:

  • Marker expression levels
  • Primary antigen: Expressed at high density, often defining lineages
  • Secondary antigen: Often expressed over a continuum
  • Tertiary antigen: Critical markers expressed at low density
  • Marker coexpression, especially of dim markers
  • The gating strategy needed to identify the population(s) of cells you wish to interrogate
 
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Step 3

Know your flow cytometer

Knowing your instrument is essential. Understanding your instrument's configuration will let you know how many markers and which fluorochromes your instrument can detect.

Elements to consider include:

  • Laser wavelength for excitation
  • Number of detectors for each laser
  • Filters available to detect the fluorochromes
 
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Step 4

Fluorochrome assignment

Carefully select fluorochromes to resolve markers at all expression levels and minimize spectral overlap. Consider using tools like a fluorochrome resolution ranking and a spectrum viewer to help assess:

  • Fluorochrome resolution
  • Cross laser excitation
  • Fluorochrome spillover
     

Remember to pair bright fluorochromes with low expressing antigens and dim fluorochromes with high expressors. Keep in mind that spread only impacts the resolution of coexpressed markers.

 
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Step 5

Review panel

Review your panel design and begin ordering your reagents. Remember to titrate your mass size reagents and optimize your staining protocol. Include proper controls for compensation, FMO and biological controls to help ensure optimal panel performance.

 

To find more panel design tips and some fun facts, download the “Flow cytometry panel design journey” infographic.

 

Download Now
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Videos
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Multicolor flow cytometry panel design videos

Add A Solid Foundation for Simpler and Smarter Panel Design

A comprehensive overview of panel design fundamentals and different approaches to simplify panel design.

Flow Cytometry Instrument Characterization and Set Up for Optimal Panel Design

This video explains how to leverage flow cytometry configurations to help maximize resolution of populations of interest.

 
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Avoiding Resolution Loss When Using Fix and Permeabilization Buffers for Intracellular Staining

In this video you will learn helpful strategies to help prevent loss of resolution due to intracellular fixation and permeabilization buffers.

 
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Understanding and Managing Fluorescence Spillover

In this video you will learn how to manage fluorescence spillover to get the most out of your flow cytometry experiments.

 
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Relationship Between Fluorescence Spillover and Spread

This video will help you understand the relationship between florescence spillover and spread to help you implement the right strategies to resolve your populations of interest.

 
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Minimizing the Impact of Spread in Flow Cytometry Experiments

This video provides strategies to help minimize the impact of spread in flow cytometry experiments to help improve resolution.

 
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Panel Design Workflow for Optimal Fluorochrome-Antigen Matching

This video provides simple strategies for fluorochrome-antigen matching to help prevent the introduction of spread and subsequent resolution loss.

 
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BD Horizon™ Tour Series
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BD Horizon™ Tour Series

Achieve: Putting It All Together: Panel Design Principles for Surface and Intracelluar Staining

This webinar explores concepts, best practices and available tools to help you efficiently navigate multicolor flow cytometry.

 

Speaker

Andrew D. Bantly

Technical Applications Specialist

Watch Now
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Sentinel Marker Approach to Multicolor Flow Cytometry: An Experimental Design that Uses Key Markers to Define Cell Subpopulations to Extend Instrument Capability

Discover a new way of looking at fluorochromes and markers that can maximize the number of parameters achievable on any instrument.

Speaker

Bob Balderas, MBA

VP Biological Sciences & VP Market Development

BD Life Sciences–Biosciences

Watch Now
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Resolve: Managing Instrument Setup to Address Fluorescence Spillover and to Maximize Resolution

This webinar offers a comprehensive look at best practices for managing instrument set up to help you maximize your instrument’s parameters while minimizing spillover and resolution loss. 

Speaker

Alan Stall

Principle Scientist 

BD Life Sciences–Biosciences

Watch Now
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Elevate: The Importance of Surface Antigen Density and Intracellular Epitope Availability in Choosing the Appropriate Fluorochrome/Antibody Combination

This webinar explores the importance of understanding antigen density (the number of cell surface receptors on a cell) in relation to antibody/fluorochrome combinations for optimal panel design. 
 

Speaker 

Bob Balderas, MBA

VP Biological Sciences & VP Market Development

BD Life Sciences–Biosciences

 

Watch Now
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Reveal: Implications of Relative Fluorochrome Brightness in Resolving the Population of Interest

This webinar explores the journey to finding what nature is hiding using flow cytometry by understanding the biology of your cells and the relative brightness of fluorochromes. 

Speaker

Bob Balderas, MBA

VP Biological Sciences & VP Market Development

BD Life Sciences–Biosciences

Watch Now

Watch Now
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BD Harmony Series
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BD Harmony Series

Ask the Experts—A Solid Foundation for Simpler and Smarter Panel Design

This webinar offers viewers practical strategies for designing optimized multicolor flow cytometry panels by addressing frequently asked questions. 
 

Speakers

Bob Balderas, MBA

VP Biological Sciences & VP Market Development

BD Life Sciences–Biosciences


Mirko Corselli, PhD

Global Scientific Content Manager

BD Life Sciences–Biosciences


Rui Gardner, PhD

Head of Flow Cytometry Core Facility

Memorial Sloan Kettering Cancer Center


Yolanda Mahnke, PhD

Founder

FlowKnowHow LLC

Watch Now
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Providing a Solid Foundation for Simpler Smarter Flow Cytometry Panel Design: Harmony Seminar Series

This webinar is part of the Harmony Series and offers viewers panel design best practices, with emphasis on spillover and identification of optimal fluorochrome combinations to simplify panel design.

Speaker

Mirko Corselli, PhD

Global Scientific Content Manager

Research Solutions, BD Life Sciences–Biosciences

Watch Now
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A Solid Foundation for Simpler and Smarter Panel Design

This webinar explores strategies to help customers create a solid chromatic foundation for multicolor panel design
  

Speakers

Bob Balderas, MBA

VP Biological Sciences & VP Market Development

BD Life Sciences–Biosciences

Watch Now
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Other

BD Panel Design Matters: Practical Aspects of Designing Flow Cytometry Panels

This webinar explores strategies for minimizing flow cytometry panel design pain points as well as panel optimization
 

Speaker

Alan Stall

BD Fellow, Principal Scientist, BD Life Sciences–Biosciences

Watch Now
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Making Panel Design Easier in the Era of High-Dimensional Flow Cytometry

This webinar offers comprehensive strategies for adding efficiency to the flow cytometry panel design process

Speaker

Anis Larbi, PhD

Head of A*STAR Flow Cytometry Facility, Immuno-monitoring Platform and Principal Investigator, Biology of Aging Program 
Singapore Immunology Network (SIgN)

Watch Now
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Compensation Matters: Considerations When Designing Your Flow Cytometry Panels

This webinar provides a robust overview on compensation best practices to help achieve your resolution goals. 

Speaker

Alan Stall

BD Fellow, Principal Scientist, BD Life Sciences–Biosciences

Watch Now
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Resources
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PUBLICATIONS
  • Mahnke YD, Roederer M. Optimizing a multicolor immunophenotyping assay. Clin Lab Med. 2007;27(3): 469–485, v. doi: 10.1016/j.cll.2007.05.002

  • Mair F, Tyznik A. High-dimensional immunophenotyping with fluorescence-based cytometry: a practical guidebook. Methods Mol Biol. 2019;2032:1-29. doi: 10.1007/978-1-4939-9650-6_1

  • Nguyen R, Perfetto S, Mahnke YD, Chattopadhyay P, Roederer M. Quantifying spillover spreading for comparing instrument performance and aiding in multicolor panel design. Cytometry A. 2013;83(3):306-315. doi: 10.1002/cyto.a.22251

  • Roederer M. Spectral compensation for flow cytometry: visualization artifacts, limitations, and caveats. Cytometry. 2001;45(3):194-205. doi: 10.1002/1097-0320(20011101)45:3<194::aid-cyto1163>3.0.co;2-c 

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For Professionals in Research

For Research Use Only. Not for use in diagnostic or therapeutic procedures.

Class 1 Laser Product.

Refer to manufacturer's instructions for use and related User Manuals and Technical Data Sheets before using this product as described.

Comparisons, where applicable, are made against older BD technology, manual methods or are general performance claims. Comparisons are not made against non-BD technologies, unless otherwise noted.