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TR-1003-G Sigma-AldrichPolybrene Infection / Transfection Reagent

A highly efficient method of gene transfer into mammalian cells leveraging infection with retroviral vectors.

Polybrene Infection / Transfection Reagent MSDS (material safety data sheet) or SDS, CoA and CoQ, dossiers, brochures and other available documents.

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TR-1003-G

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Description
Catalogue Number	TR-1003-G
Trade Name	Specialty Media
Description	Polybrene Infection / Transfection Reagent
Overview	A highly efficient method of gene trasfer into mammalian cells is through infection with retroviral vectors. The efficiency of retroviral infection is enhanced significantly, 100 to 1,000 fold in some cells, by including polybrene during the infection. Polybrene with DMSO shock is also used to mediate DNA transfer into a variety of cell types, such as: CHO, chicken embryo fibroblases, NIH3T3 cells, and myeloid cells.

References

Product Information
Presentation	10mg polybrene per mL sterile Ultra Pure water.
Quality Level	MQ100

Applications
Application	A highly efficient method of gene transfer into mammalian cells leveraging infection with retroviral vectors.
Application Notes	A highly efficient method of gene transfer into mammalian cell is through infection with retroviral vectors. The efficiency of retroviral infection is enhanced significantly, 100 to 1,000 fold in some cells, by including polybrene during the infection. Polybrene with a DMSO shock is also used to mediate DNA transfer into a variety of cell types, such as CHO, chicken embryo fibroblasts, NINH-3T3 and Myeloid cells. Protocol: Retroviral Infection Recombinant retroviral stocks are prepared by adding 5mls of growth medium with 5% serum to a near confluent monolayer of transfected retroviral packaging cells in a 100mm plate. After 24 hours the medium is removed and filtered through a 0.45um filter. Cells to be infected with this recombinant retroviral stock are plated at 500,000 cells per 100mm plate in 10mls of complete medium. 24 hours later, remove the growth medium from the cells. Infect cells with 2mls of the viral supernatant (or a dilution of the virus stock into 2mls) in the presence of 5ug to 10ug of polybrene per ml (final concentration). Incubate cells for 3 to 6 hours at 37°C. Add 8mls of complete medium. Three days after infection, split the cells 1:5 into selection medium. References: Toyoshima, K. and Vogt, P.K., 1969. Virology. 38:414-426 Coelen, J.R., Jose, D.G. and May, J.T. 1983. Arch. Virol. 75:307-311 Protocol: Transfection Plate cells at approximately 50% confluence in complete growth medium. 18 to 24 hours post plating, prepare the DNA-Medium-Polybrene solution, immediately before using as follows: Note: Each component must be added in the proper sequence. 1st: Complete growth medium (2mls for a 60mm plate and 3mls for a 100mm plate) warmed to 37°C. 2nd: Plasmid DNA, 10ng to 10ug. Gently mix. 3rd: Polybrene to a final concentration of 5ug to 10ug per ml. Gently mix Remove medium from plate and add DNA-Medium-Polybrene solution to cells. Incubate cells at 37°C for 6 to 20 hours with occasional gentle rocking approximately every 1.5 hours for the first 6 hours. Remove DNA-Medium-Polybrene solution and gently overlay cells with DMSO shock solution (15% DMSO in 1X HBSS: Specialty Media catalog #S-051-D) 3mls per 60mm dish and 4mls per 100mm plate. Manually rock the dish for 10 seconds to evenly distribute the solution, and then incubate the cells for exactly 4 minutes at 37°C. Immediately remove the DMSO shock solution and gently rinse the cells twice with complete growth medium, 5mls per wash per 60mm dish, 10mls per wash per 100mm dish Add complete growth medium to the cells. For Stable transformants, remove the growth media and split the cells 1:5 into selection medium. For transient expression, remove the growth medium and add fresh growth medium. Harvest cells and/or medium after 24 to 72 hours. References: Chaney, W.G. et al., 1986. Somatic Cell and Molecular Genetics. Vol. 12, No. 23, 237-244. Aubin, R.J. et al. 1988. Somatic Cell and Molecular Genetics. Vol. 14, No. 2, 155-167. Chisholm, O. et al., 1998. Nucleic Acids Research. Vol. 16, No. 5, 2352 Reagent is supplied filtered through 0.2um membranes and hydrated with sterile H20.

Applications

Application

A highly efficient method of gene transfer into mammalian cells leveraging infection with retroviral vectors.

Application Notes

A highly efficient method of gene transfer into mammalian cell is through infection with retroviral vectors. The efficiency of retroviral infection is enhanced significantly, 100 to 1,000 fold in some cells, by including polybrene during the infection. Polybrene with a DMSO shock is also used to mediate DNA transfer into a variety of cell types, such as CHO, chicken embryo fibroblasts, NINH-3T3 and Myeloid cells.

Protocol: Retroviral Infection

Recombinant retroviral stocks are prepared by adding 5mls of growth medium with 5% serum to a near confluent monolayer of transfected retroviral packaging cells in a 100mm plate. After 24 hours the medium is removed and filtered through a 0.45um filter.

Cells to be infected with this recombinant retroviral stock are plated at 500,000 cells per 100mm plate in 10mls of complete medium.

24 hours later, remove the growth medium from the cells. Infect cells with 2mls of the viral supernatant (or a dilution of the virus stock into 2mls) in the presence of 5ug to 10ug of polybrene per ml (final concentration). Incubate cells for 3 to 6 hours at 37°C.

Add 8mls of complete medium. Three days after infection, split the cells 1:5 into selection medium.

References:

Toyoshima, K. and Vogt, P.K., 1969. Virology. 38:414-426

Coelen, J.R., Jose, D.G. and May, J.T. 1983. Arch. Virol. 75:307-311

Protocol: Transfection

Plate cells at approximately 50% confluence in complete growth medium.

18 to 24 hours post plating, prepare the DNA-Medium-Polybrene solution, immediately before using as follows:

Note: Each component must be added in the proper sequence.

1st: Complete growth medium (2mls for a 60mm plate and 3mls for

a 100mm plate) warmed to 37°C.

2nd: Plasmid DNA, 10ng to 10ug. Gently mix.

3rd: Polybrene to a final concentration of 5ug to 10ug per ml. Gently mix

Remove medium from plate and add DNA-Medium-Polybrene solution to cells. Incubate cells at 37°C for 6 to 20 hours with occasional gentle rocking approximately every 1.5 hours for the first 6 hours.

Remove DNA-Medium-Polybrene solution and gently overlay cells with DMSO shock solution (15% DMSO in 1X HBSS: Specialty Media catalog #S-051-D) 3mls per 60mm dish and 4mls per 100mm plate. Manually rock the dish for 10 seconds to evenly distribute the solution, and then incubate the cells for exactly 4 minutes at 37°C.

Immediately remove the DMSO shock solution and gently rinse the cells twice with complete growth medium, 5mls per wash per 60mm dish, 10mls per wash per 100mm dish

Add complete growth medium to the cells.

For Stable transformants, remove the growth media and split the cells 1:5 into selection medium.

For transient expression, remove the growth medium and add fresh growth medium. Harvest cells and/or medium after 24 to 72 hours.

References:

Chaney, W.G. et al., 1986. Somatic Cell and Molecular Genetics. Vol. 12, No. 23,

237-244.

Aubin, R.J. et al. 1988. Somatic Cell and Molecular Genetics. Vol. 14, No. 2, 155-167.

Chisholm, O. et al., 1998. Nucleic Acids Research. Vol. 16, No. 5, 2352

Reagent is supplied filtered through 0.2um membranes and hydrated with sterile H20.

Biological Information
Media Form	Liquid
Stem Cell Type	Mouse Embryonic Stem Cells

Physicochemical Information

Dimensions

Materials Information

Toxicological Information

Safety Information according to GHS

Safety Information

Product Usage Statements
Usage Statement	Unless otherwise stated in our catalog or other company documentation accompanying the product(s), our products are intended for research use only and are not to be used for any other purpose, which includes but is not limited to, unauthorized commercial uses, in vitro diagnostic uses, ex vivo or in vivo therapeutic uses or any type of consumption or application to humans or animals.

Storage and Shipping Information
Storage Conditions	Store at -20°C upto 2 years.

Packaging Information
Material Size	1 mL

Transport Information

Supplemental Information

Specifications

Global Trade Item Number
Catalog Number	GTIN
TR-1003-G	04053252398025

Documentation

Polybrene Infection / Transfection Reagent SDS

Title
Safety Data Sheet (SDS)

Polybrene Infection / Transfection Reagent Certificates of Analysis

Title	Lot Number
Polybrene Transfection Reagent - 3488247	3488247

References

Reference overview	Pub Med ID
Using small molecules to improve generation of induced pluripotent stem cells from somatic cells Desponts C. & Ding S. Methods Mol. Biol. 636 207-218 2010 Show Abstract Induction of pluripotent stem cells from somatic cells by defined factors was shown to be possible only recently, but already several laboratories have made tremendous strive toward improving and understanding the process. Originally, Oct4, Sox2, Klf4, and cMyc were identified as being the combination of genes necessary to induce reprogramming. It was later shown that cMyc was dispensable; however, in its absence the process was less efficient and took a considerably longer period of time to occur. Furthermore, others have shown that the combination of Oct4, Sox2, Nanog, and Lin28 could also induce reprogramming. One major caveat associated with these techniques remains the need for overexpression of several genes using viral systems. Until very recently, most studies were done using integrating viruses such as retroviruses and lentiviruses. This method ensured that the protein of interested would be expressed at a high concentration and for an adequate period of time necessary to induce reprogramming. Up to date, others have now been able to use different nonintegrative method such as adenovirus and plasmid transfection to induce reprogramming. Furthermore, piggyBac transposition was successfully used to induce reprogramming of murine cells. Most importantly, it was recently published that reprogramming can be induced in the absence of virus, with proteins and small molecules. All of the later methods are appealing since they do not require the integration of the virus or plasmid to exert its effect. However, one avenue that would be all the more therapeutically appealing would be to induce reprogramming in the absence of gene overexpression systems, using small molecules to modulate signaling pathways in the somatic cells. A few molecules have already been identified with the ability to either improve the process or replace one or two of the genes deemed necessary for reprogramming. We have screened successfully for compounds that can replace some of these factors, and share the methods developed following these screens.	20336525

Reference overview

Pub Med ID

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TR-1003-G Sigma-AldrichPolybrene Infection / Transfection Reagent

A highly efficient method of gene transfer into mammalian cells leveraging infection with retroviral vectors.

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Overview

Documentation

Polybrene Infection / Transfection Reagent SDS

Polybrene Infection / Transfection Reagent Certificates of Analysis

References

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