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CL-2™ RUO

Catalogue No.

CL-2™ RUO
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  • Description
  • Graph Details

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MaxCyte

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Catalogue No.

CL-2™ RUO

CL-2™ RUO

Large-scale RUO Processing Assemblies
Flow Electroporation processing assemblies for research applications in large-volume scales

Research Use Only (RUO) Flow Electroporation Processing Assemblies enable the discovery and development of applications at large-scales. These flow electroporation consumables are made from high-grade, inert materials to protect precious cells. They include additional design features for easy sample loading and recovery and closed process adaptability.

CL-2™ RUO

  • Shake flask to bioreactor production scales
  • Bioweld compatible; closed process adaptable
  • Enables processing of up to 20 billion cells in 30 minutes

Configuration:Closed system, PVC bags & tubing with luer locking syringe ports
Cell Range:5×107– 2×1010
Volume Range:10 – 100 mL
Application:Research Use Only
Catalog:SCL-2

Compatible with STx™

Download Catalogue
Request a Quote
  • Description
  • Graph Details
Description icon

Large-scale RUO Processing Assemblies
Flow Electroporation processing assemblies for research applications in large-volume scales

Research Use Only (RUO) Flow Electroporation Processing Assemblies enable the discovery and development of applications at large-scales. These flow electroporation consumables are made from high-grade, inert materials to protect precious cells. They include additional design features for easy sample loading and recovery and closed process adaptability.

CL-2™ RUO

  • Shake flask to bioreactor production scales
  • Bioweld compatible; closed process adaptable
  • Enables processing of up to 20 billion cells in 30 minutes

Configuration:Closed system, PVC bags & tubing with luer locking syringe ports
Cell Range:5×107– 2×1010
Volume Range:10 – 100 mL
Application:Research Use Only
Catalog:SCL-2

Compatible with STx™

Graph Details icon

CL-2-Efficiency-FITC@2x

Graph Details: HEK293F cells were suspended in MaxCyte® Electroporation Buffer with FITC-conjugated dextran and divided into 6 CL-2 PAs. Samples were transfected on two separate GTx™ Instruments (3 each). Three aliquots were taken from each CL-2 post electroporation and assayed for fluorescence.

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