Transfection methods and techniques altogen biosystems. Electroporation parameters for dna plasmids 15kb using. Establishing transfection methods that enable highly efficient dna uptake has become increasingly important. The common causes of transfection failure are decrease transfection efficiency and decreased cell viability. For large plasmids, it is important to prepare a highly concentrated solution of the plasmid for electroporation. Optimization of gene transfection in murine myeloma cell. Transfection guide overview of transfection methods. Madison, wi, march 8, 2011 in addition to reliable high efficiency transfection reagents, mirus bio has expanded its transfection expertise with the development of the reagent agent a new online tool designed to determine the best solution for delivery of any nucleic acid into any cell type, including hardtotransfect. Btw for b cell electroporation, including b cell in the pbmc fraction or cd40l expanded b cells, electroporation works best with celetrix electroporation system at about 80% efficiency, much. The neon transfection system offers open and transparent protocols that are optimized for ease of use. Using neon pipette and tip, transfect 10ul of cell rna mixture.
Starrlab electroporation using neon electroporation from. Neon transfection system thermo fisher scientific pw. Protocol overview i electroporated 5 million cells with 4 ug of a gfp plasmid using the neon transfection system 100 l kit. Efficient electroporation with neon transfection system. A free program designed to help you achieve your scientific aspirations. Press the pushbutton on the neon pipette down to the first stop, immerse in the celldna mixture and slowly release the pushbutton to suck up 100 l of celldna mixture. All available information is shown in the detailed view. Transfection protocols vary based on cell type to be transfected, transfection method, and transfection reagent.
Efficiencyup to 90% transfection and geneediting efficiency in extremely difficult cells, including immune, primary and stem cells. Invitrogen neon transfection system vxmpk5000s duration. Neon transfection of primary mouse t cells the ansel lab. Request a sample for low toxicity transfection mirus bio. For detailed instructions, refer to the manual supplied with the product or download the manual from. Cloned genes can be transfected into cells for biochemical characterization, mutational analyses, investigation of the effects of gene expression on cell. Reverse transfection is defined as the process of adding the encapsulated cargo molecule plasmid dna, sirna, mirna while simultaneously plating the cells. Cell type specificity and structural determinants of ires activity from. The hyperlinked cell line names take you to a pdf that gives. This device allows you to transfection directly in the pipette tip, limiting the steps required. Search for publications in the transfection database with polyplus transfection reagents or for transfection conditions.
Flow cytometric data were analyzed using the program, expo32adc. The insertion of dna into a cell enables the expression, or production, of proteins using the cells own machinery, whereas insertion of rna into a cell. Thermofisher neon transfection system 10 l kit mpk1025. Our universal transfection reagent is a unique formulation of a proprietary polymer blend. Fast and easy protocol is compatible with serum, serumfree medium and antibiotics. The flexible and open system allows the user to perform highquality transfections using optimized or userdefined protocols in three simple steps with as few as 2 x 10 4 cells. Monitor the needle to make sure there are no sparks arcing, which will ruin the transfection. In practical terms, reverse transfection refers to cell based array experiments in which cells are pipetted onto preplated cargo molecules.
Oncogenic gene fusion fgfr3tacc3 is regulated by tyrosine. At this point i have a set of tubes with cells and appropriate rna combined. Very important to make sure that there are no bubbles in the tip. Established cell lines, stem cells, primary cells, hardtotransfect cells. Ncbi gene expression omnibus database under accession number. Product overview the 384well nucleofector tm system is an independent platform for highthroughput nucleofection in a 384well format. Any gaps between the pipette tip and the pipette will cause poor transfection. Transfection efficiency and survival rate achieved. Animal originfree, serumfree and designed specifically for use with the neon transfection system.
The development of reporter gene systems and selection methods for stable maintenance. Transfection efficiency testing using fluorescenceactivated cell sorting. Typically, 24 to 48 hours between transfection and. Invitrogen neon transfection system starter pack 1 pack. Mouse myeloma cell lines sp20, ns0, ns1, ag8, and p3u1 were transfected with pegfpn1 vector using lipofectamine 2000, jetpei and lyovec commercial transfection reagents in different combinations. An electroporation protocol for efficient dna transfection. During the optimization process, a range of conditions for different transfection parameters dna concentration, number of cells, pulse settings was tested.
The neon transfection system uses a single transfection kit neon kit that is compatible with various mammalian cell types including primary and stem cells thereby avoiding the need to determine an optimal buffer for each cell type. Sigmas universal transfection reagent is a unique formulation of a proprietary polymer blend used for transient and stable transfection of nucleic acids into various eukaryotic cell lines and hardto. Established cell lines, hardtotransfect cells, primary cells, stem cells. For use with the neon transfection system use this kit for transfection volumes of 100l, containing 5 x 10 5 2 x 10 6 adherent cells or 1 x 10 6 5 x 10 6 suspension cells cells that have been transfected using the included 100l neon tips are then ready to be washed and plated into a 6well, 60mm, or 10cm culture dish, depending on protocol. L, containing 5 x 10 42 x 10 5 adherent cells or 1 x 10 65 x 10 5 suspension cells.
Transfection the delivery of dna or rna into eukaryotic cells is a powerful tool used to study and control gene expression. Jul 12, 20 a wide variety of mammalian cell types is used in gene transfection studies. All mass spectra from were analyzed with maxquant software version. Transfection guide overview of transfection methods promega. The neon transfection system enables fast and efficient delivery of nucleic acids. This device have an electrode in the tip, increasing the rate of viability of cells and the % of transfection. Invitrogen neon transfection system mpk5000 electroporation. Neon transfection system instructions for using the neon transfection system for transfection of mammalian cells are described below. Neon transfection system protocols and cell line data thermo. The table below contains a listing of the cell lines and primary cells successfully electroporated with the neon transfection system or the predecessor instrument the microporator mp100. Plate cells to obtain 7080% cell density on the day of transfection. As always, qiagen cannot verify data supplied from outside sources. Universal transfection reagent protocol sigmaaldrich. Cells were transfected using the neon electroporation system.
Highefficiency genomic editing in epsteinbarr virustransformed. Cloned genes can be transfected into cells for biochemical characterization, mutational analyses, investigation of the effects of gene expression on cell growth, investigation of gene regulatory elements, and to produce a specific protein. Has anybody done transfection of b lymphocytes using neon. Neon transfection system cell line data thermo fisher. Cells that have been transfected using the included 10 l neon tips are rea.
A costeffective approach to microporate mammalian cells with. Transfection cell database our searchable database contains data from researchers like yourself who have shared their experimental results with us. Using various chemical or physical methods, this gene transfer technology enables the study of gene function and protein expression in a cellular environment. Typically, 24 to 48 hours between transfection and activity assay is sufficient. Altogen cro offers in vivo rnai services, tumor xenograft models, toxicology testing, stable cell line generation, and. Neon transfection system thermo fisher scientific us. Neon transfection system thermo fisher scientific es. Invitrogen neon transfection system 100 l kit 96 x 2.
High transfection efficiency of jurkat cells with life technologies neon tranfection system. With an extremely fast plate processing time of 1 minute per plate. Piggybac transposonmediated gene delivery efficiently generates. I followed the manufacturers online protocol for 3t3l1 cells. Use the table below to troubleshoot transfection experimental failure. Transfection is the process of inserting genetic material, such as dna and double stranded rna, into mammalian cells. Efficient, highthroughput transfection of human embryonic. Electroporation parameters for dna plasmids 15kb using the. Neon transfection system enables fast and efficient delivery of nucleic acids into all mammalian cell types, including primary, stem, and difficulttotransfect cells. Remove the pipette from the station and gently expel the cell dna mixture by. Transfected hek293 cells were collected, washed once in pbs, and lysed.
A costeffective approach to microporate mammalian cells. Msms spectra were searched against the crap protein sequence database. For example, vary the concentration of trans itlt1 reagent from 28. Aug 31, 20 the very basic requirement for the existence of genetic engineering is a simple fact. The very basic requirement for the existence of genetic engineering is a simple fact. Use this selection table to find the neon transfection system electroporation conditions, transfection efficiency and survival rate and microscopy images of cells. The underlying reason is that this method, which employs electrical pulses to create transient pores in cell membranes, reproducibly yields high transfection. Gibco 24 hours of stem cells virtual event presented by.
The optimal time period depends on the protein being expressed, and thus the sensitivity of the assay. With an extremely fast plate processing time of 1 minute per plate, it is perfectly suited for screening applications with maximum reproducibility. For detailed instructions, refer to the manual supplied with the. Some cells, like hela cells, are easy to transfect with lipid reagents. Mar 03, 2015 invitrogen neon transfection system mpk5000 electroporation lot 551. The insertion of dna into a cell enables the expression, or production, of proteins using the cells own machinery, whereas insertion of rna into a cell is used to downregulate the production of a specific protein by stopping translation. Both systems can result in the efficient transfection of hesc. Neon electroporation transfection neon transfection system cell line data the table below contains a listing of the cell lines and primary cells successfully electroporated with the neon transfection system or the predecessor instrument the microporator mp100. A wide variety of mammalian cell types is used in gene transfection studies. Optimize dna transfection transfection, electroporation and.
While the neon system had a higher transfection efficiency, it also had increased variability between multiple transfections 36. Protocol for electroporation of cas12a ribonucleoprotein rnp into. Neon transfection system cell line data thermo fisher scientific. Cells that have been transfected using included 10. Neon electroporation transfection thermo fisher scientific us. Reagent agent transfection database from the transfection.
The neon system employs specialized consumable pipette tips containing goldplated electrodes as electroporation chamber. If the medium becomes very dense with cell debris, change to fresh antibiotic medium after 47 d. Jackie webb scientist i, thermo fisher scientific speaker. The neon 10 l transfection system draws 10 l of cells and transfection. Broad spectrum dna delivery achieve high expression in many cell types, including hard to transfect cell lines. Some of the transfection efficiency and viability data was generated with the microporator mp100, the predecessor or the neon transfection system see. Transfection of mammalian cells with fluorescent protein. Monitor the progress of the transfection every few days by observing the amount of cell death and the color of the culture medium. Transfection of mammalian cells with fluorescent protein fusions. An electroporation protocol for efficient dna transfection in. Over 4000 publications, cell lines and primary cells available.
Transfection reagents are highly efficient for dna and sirna transfection in vivo and in vitro. I will start by giving you an overview of the topics that i will cover during todays webinar. The neon transfection system 10 l kit is designed specifically for use with the. Altogen cro offers in vivo rnai services, tumor xenograft models, toxicology testing, stable cell. I followed the manufacturers online protocol for 3t3l1 cells 1,300v, 20 ms, 2 pulses. Intracellular uptake of reporter vector encoded with egfp at 24 hr following transfection of jurkat cells with neon transfection system. Neon transfection system 10 l kit thermo fisher scientific. With the introduction of new systems for transfection such as the neon transfection system. Neon transfection system feb232010 hello, we think of acquiring soon a new transfection system from invitrogen, the neon. General information about the cell line or primary cell. Request a free sample of low toxicity transfection reagents. Apr 30, 2019 nk92 cell line, freshly isolated resting or il2activated nk cells were electroporated with the neon transfection system thermo fisher scientific, waltham, massachusetts, usa. Cell transfection database polyplustransfection expertise.
Invitrogen neon transfection system starter pack life. Altogen biosystems provides in vivo transfection reagents, over 100 preoptimized in vitro transfection kits for cell lines and primary cells, and electroporation delivery products. A variety of viral and nonviral delivery systems have been developed, but electroporation is often the selected method of choice. Optimize dna transfection transfection, electroporation. Transfection is the process of introducing nucleic acids into eukaryotic cells by nonviral methods. Nk92 cell line, freshly isolated resting or il2activated nk cells were electroporated with the neon transfection system thermo fisher scientific, waltham, massachusetts, usa. The manufacturer typically has a database with a recommended setting for a given cell. During the optimization process, a range of conditions for different transfection.
Jun, 2010 transfection is a powerful analytical tool enabling study of the function of genes and gene products in cells. Transfection of h9 is efficient and the resulting cells have a high viability. Transfection is a powerful analytical tool enabling study of the function of genes and gene products in cells. Fortebio octet qk labelfree analyzer with computer and octet software lot 400. Using neon pipette and tip, transfect 10ul of cell. The transfection methods are broadly classified into three groups. Reagent agent transfection database from the transfection experts. Cell applications, inc 5820 oberlin drive, suite 101 san diego, ca 92121 open mf, 8am5pm pst. Get improved transfection outcomes with the neon transfection system. When working with a new cell type, test a range of reagent volumes at a fixed dna amount to find the level that achieves the highest transfection efficiency with minimal toxicity. Pc12 is an established rat pheochromocytoma cell line, which responds to exposure to ngf with cessation of growth, expression of cytoplasmic processes, and differentiation into cells resembling sympathetic.
Get highly efficient transfection of primary cells, stem cells, and difficultto transfect cells with the versatile and easytouse neon transfection system. Unfortunately, no single delivery method or transfection reagent can be applied to all types of cells. Little is known about transfectability of murine myeloma cell lines by different transfection reagents. The basic, single cuvette based nucleofector tm system for efficient transfection of hardtotransfect cell lines and primary cells with different substrates e. In general, the use of such a capillary electroporation system which is often called a microporation device has important advantages compared with conventional cuvettebased electroporation chambers. As a bit of background, transfection is a method to transfer genetic material into cells in order to add or alter the expression of a specific gene in a cell.
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