General protocol for recovering or freezing primary cells. Gently pipette up and down to create a single cell suspension using a 10ml pipette. Following electroporation, b cells were plated onto the op9 or op9 baffcd40l stroma. Systemic human ilc precursors provide a substrate for tissue ilc differentiation. When using accutase, cells can be plated directly into culture vessel without centrifuging to pellet cells as long as accutase is inactivated by the addition of the. Next, we examined whether our twostage protocol for nk cell production is applicable to these pbcipsc lines.
Note that cell culture conditions vary for each cell type. Jan 15, 2005 human embryonic stem hes cells represent a unique population of cells capable of selfrenewal and differentiation. Any and all media, supplements, and reagents must be sterilized by filtration through a 0. The manufacturers protocol was followed with the following exception. Using the parental op9 line and 4 clonal populations we tested. Cell culture guidelines the following is a general guideline for culturing of cell lines. Once matrigel matrix is thawed, swirl vial to ensure the material is dispersed.
Op9 feeder cells are superior to m210b4 cells for the. In this paper, we describe a protocol for hematopoietic differentiation of human pluripotent stem cells hpscs and generation of mature myeloid cells from hpscs through expansion and. The lowest moi at which all cells or enough cells for the specific approach. This article contains a series of protocols, the first of which describes the establishment, maintenance, and storage of op9 and op9 dl1 cells. In this co culture system, es cells differentiate, into hemangioblasts at day5, when placed on a confluent layer of mstrawberry op9 cells. The cell samples were used in a standard colonyformation assay. After 1012 days of culture on op9 cells, hzs were picked up under microscopic inspection using a small scalpel and pipette. Atcc offers custom testing services for mycoplasma detection and human cell line authentication str analysis. The third method of op9 differentiation, io, employs low serum. The op9, a stromal cell line from mouse bone marrow, has hematopoietic supportive capacity. Culture protocols, which resides in the highly useful methods in molecular biology series, to be a major resource of information for their research projects.
Part c provides a protocol for preparing a midlog culture of e. To study the effect of op9 cells on the proliferation potential of. Pluripotent stem cells as source of dendritic cells for. For more information on enzymatic dissociation and subculturing of cell lines consult chapter in. To initiate differentiation, undifferentiated es cells were suspended in amem supplemented with 20% fetal calf serum fcs and seeded onto op9 cell layers. The standard es op9 co culture protocol entails the placement of es cells onto a confluent layer of op9 cells. One 10cm plate of a two day culture will make three 6 well plates or four 24 well plates. Heidcamp, gustavus adolphus college a large collection of protocols related to cell biology work from microscopy to cell culture, histochemistry, etc. T lineage differentiation from human embryonic stem cells. Megakaryocytic differentiation of mouse embryonic stem cells. Differentiation of mouse embryonic stem cells escs or hematopoietic stem cells hscs from fetal liver or bone marrow into tlymphocytes can be achieved in vitro with the support of op9 dl1 cells, a bonemarrowderived stromal cell line that ectopically expresses the notch ligand, deltalike 1 dll1. Thank you for your understanding, patience and flexibility as atcc does everything it can to help reduce the impact of. Remove a volume of the single cell suspension and dilute with trypan blue solution and magnetic cell sorting buffer macs buffer for counting. Characterization of op9 as authentic mesenchymal stem cell line.
The protocol begins with an overnight suspension culture. Cells in midlog growth can generally be rendered more competent to uptake plasmid dna than can cells at stationary phase. Systemic human ilc precursors provide a substrate for. In vitro differentiation of hesc toward hematopoietic lineage. Op9 and m210b4 cell lines are used as feeder layers. In this chapter, we describe a threestep cell culture method for directed differentiation of human embryonic stem cells hescs to dendritic cells dcs that includes 1 hesc differentiation into hematopoietic progenitors by coculture with op9 stromal cells, 2 expansion of myeloid dc precursors in suspension bulk cultures with granulocyte.
On day 0, dilute the matrigel matrix to 5 mgml with icecold mdck complete cell culture medium. A mstrawberry op9 cell are subcultured at 7090% confluency. Animal cell culture protocol aseptic technique and good cell culture practice to ensure all cell culture procedures are performed to a standard that will prevent contamination from bacteria, fungi and mycoplasma and cross contamination with other cell lines. Secure a 6cm plate of hek293t cells from the stock incubator. Cell culture basics introduction to cell culture, covering topics such as laboratory setup, safety and aseptic technique including basic cell culture protocols and video training. Plant cell culture protocols methods in molecular biology. Among many mouse stroma cell lines, several researchers have used 35 op9 stromal cell line 6 and the derived op9dl1 7, 8, op9dl4 9 stromal cell lines for coculturing. Acquire pictures of the cells by fluorescence microscopy after 24 and 48 hours. Furthermore, current protocols involve evaluating only the hematopoietic cells found in suspension and are not optimized for evaluation of esderived.
Cell culture applications resources including application notes and protocols to create an ideal environment for growing cells, right from the start. In the thymus, t cells are generated from hematopoietic stem cell hscderived lymphoid progenitors, which can also give rise to b cells and natural killer nk cells. For 2d hydrogel coating culture and 3d cell culture, both vitrogel 3drgd and vitrogel rgdplus were used, according to the user handbook, as described below. The es op9 co culture system was originally designed to produce hematopoietic progeny, without the over production of macrophages, as the op9 stromal cell line is derived from the calvaria of osteopetrosis mutant mice that lack functional mcsf. Midlog cells are used in the classic transformation protocol described in laboratory 10. For the op9 assay, alpha mem media is used containing 15% fbs. Addition of a cytoprotective polymer poloxamer 188 to the culture medium of late stage erythroid cells has been shown to enhance survival of. Protocol for hela cell culture and plasmid transfection av. Hood regulations a close hood sash to proper position to maintain laminar air flow b avoid. Minimum leakage if any must occur during perfusion. Cell generation from adult, embryonic, and induced. Maintenance of op9 cells op9 medium minimum essential medium alpha. A cell culture system has been established in which mouse embryonic stem cells mesc are differentiated to t cells in vitro. Very large cells tend to appear after overgrowth and these cells are a warning sign that the op9 cells will not support the maintenance of hematopoietic cells.
All cell culture must be undertaken in microbiological safety cabinet using aseptic technique to ensure sterility. Most of these pbcipscnk cells have a kirnegative phenotype, which has an interesting implication for their clinical use. All culture incubations should be performed in a humidi. Gao j1, yan xl, li r, liu y, he w, sun s, zhang y, liu b, xiong j, mao n. An average of 2 105 hesc were incubated per well of a sixwell plate. Mouse embryonic stem cell culturing protocols 4 of 6 form 105 rev b072214 7. Directed differentiation of human embryonic stem cells to. Protocol for adenoviral transduction of human cells. This application protocol describes how to handle icell neurons for use on. Add required amount of prewarmed cell culture media to fresh flask. Hence, through sequential hematopoietic differentiation on op9 cells and lymphoid commitment on op9 dll1 cells, we have established a robust protocol to generate highpurity, functional, and expandable pbcipscnk cells.
Scidhu mice were biopsied on two successive occasions, and thymocytes were analyzed for expression of egfp, cd45, cd3, cd4, and cd8 by multicolor. In the op9 coculture, the peak of hematopoietic differentiation occurred at least 1 week earlier days 7 to 9 of culture when compared to the embryoid body method and s17 coculture days 15 to 22 of culture. Pdf singlecell qpcr facilitates the optimization of. In vitro generation of t lymphocytes from embryonic stem cell. Nov 15, 2015 established from the calvaria of newborn macrophage colonystimulating factor mcsfdeficient mice, op9 is a stromal cell line that used as a feeder layer to support the in vitro differentiation of pluripotent stem cells into various hematopoietic lineage cells, including granulocytes, erythrocytes, lymphocytes, and megakaryocytes. Previously, op9 cells were shown to differentiate upon treatment with insulin oleate media. Culture of hek 293293t cells charles yin last updated. Make sure to prepare enough es cells to plate onto of the mstrawberry op9 cells for day 0 es cells will be plated at 1x103 cells per cm 2 at day 0. Pdf modified es op9 coculture protocol provides enhanced. The consequences of deviating from the culture conditions required for a particular cell type can range from the expression of aberrant phenotypes to a complete failure of the cell culture. Regain access you can regain access to a recent pay per article purchase if your access period has not yet expired. In vitro systems for the study of t cell development.
Culture es cells according to standard protocol for your particular cell line. Cell culture op9 cells were maintained in alpha minimum essential medium supplemented with 10% fbs, and 1x penstrep. The proper procedure for genome editing on tissuecultured hipscs is described in this protocol. Mybook is a cheap paperback edition of the original book and will be sold at uniform, low price. If the subculture ratio is too low, the culture will not reach confluence. Procedure 1 sanitize the cabinet using 70% ethanol before commencing work. All cell culture procedures must be conducted in a biosafety cabinet.
Although protocols for manufacturing clinicalgrade car t cells. Hematopoietic differentiation and production of mature. Standard es op9 co culture protocols entail the placement of es cells onto a confluent layer op9 cells, as well as, a day 5 replating step in order to reduce old, contaminating op9 cells from cell passage. Secretory factors from op9 stromal cells delay differentiation and. Centrifuge conical tube containing cells at 1100 rpm for 2 minutes at room temperature.
Detached cells produced in culture on op9 feeder cells exp op9 a were collected on days 57 and 127 of culture. Cells were passaged when the cultures reached 8090% confluence. Cell culture on microelectrode arrays axion biosystems. Development of an op9 derived cell line as a robust model. Protocol for hela cell culture and plasmid transfection av02hela cell culture 1. Additionally, only hematopoietic cells found in suspension are removed for evaluation of esderived progeny. Differentiation of mouse embryonic stem cells escs or hematopoietic stem cells.
Development of an op9 derived cell line as a robust model to. Development of an op9 derived cell line as a robust model to rapidly study adipocyte differentiation. Induction of t cell development by deltalike 4expressing fibroblasts. Characterization of adipogenic chemicals in three different. For this purpose, the sample must be encapsulated in glissons capsula on all areas except, obviously, the edge left by the surgeon. Counting cells using a hemocytometer contents preparing the hemocytometer preparing the cell suspension counting viability preparing the hemocytometer 1. If using a glass hemocytometer and coverslip, clean with alcohol before use. Parental op9 cells and american type culture collection. Clonal op9 cell lines differentiate rapidly and with high efficiency. We selected the 120 split from a few days previous. Cell line authentication str profiling aids in the detection of misidentified, crosscontaminated, or genetically drifted cells, which invalidate research results. Do we have a workable clinical protocol for differentiating lympho.
Crisprcas9directed genome editing of cultured cells. As the co culture proceeds, hematopoietic precursors are present at day 8, while terminally differentiated hematopoietic. Corning matrigel basement membrane matrix for 3d culture. Similarly, detached cells produced in culture on c3h10t12 feeder cells exp10t12d were collected on days 60 and 4 of culture. The recommended seeding density for each lot is stated on the. Cryopreserved human ipscderived neurons axion biosystems. Mar 15, 2006 this unit describes a system for observing and modulating t cell development in vitro via the culture of entire mouse fetal thymic lobes. To study the effect of gene knockdown on adipogenesis, we created a highly efficient preadipocyte clonal op9 cell line. Additionally, only hematopoietic cells found in suspension are. Jun 07, 2011 our lab uses an in vitro es cell co culture system to model hematopoietic development. Cell culture basics handbook thermo fisher scientific.
Pdf human pluripotent stem cells hpscsop9 coculture system is a widely used hematopoietic differentiation approach. Pdf characterization of op9 as authentic mesenchymal stem cell. Wash cells briefly with hanks solution prior trypsin treatment note. Op9 atcc crl2749 mus musculus the op9 cell line was est. However, op9 is a mouse stromal cell line, and it requires absolutely. Methods are included for the isolation of fetal thymi and culture to allow for normal t cell development on either transwell plates or gelfoam sponges.
Cell culture cell culture is one of the major tools used in cellular and molecular biology, providing excellent model systems for studying the normal physiology and biochemistry of cells e. Protocols for hematopoietic differentiation of murine es. Subsequent protocols detail how to coculture the op9 and op9dl1 cells. Since two sets are required for this assay two plates of op9 cells are needed for each cell line to be tested. Do we have a workable clinical protocol for differentiating. Herein, we have demonstrated that both cell line 3t3l1 vs. The whole protocol, encompassing human ips cell preparation, autonomous. After counting the cells, seed them in the desired collagen coated cell culture plates with mhp see table 3. Jan 31, 2018 co culture with op9 cells increases proliferation potential of adult erythroid cell culture by delaying differentiation.
Derivation of t cells in vitro from mouse embryonic stem cells. Representative esmstrawberry op9 co culture flow profile. On days 56, cells were harvested using trypsinedta, reseeded onto fresh op9 cell layers, and. Determine the rate of transduced cells per well for each moi and at each time point. Characterization of op9 as authentic mesenchymal stem cell. B for proper differentiation, es cells and esderived progeny are placed onto a overly confluent layer of mstrawberry op9 cells. Subsequent protocols detail how to co culture the op9 and op9 dl1 cells with either escs or hscs from fetal liver or bone marrow, leading to in vitro differentiation of the stem cells into lymphocytes. Modified es op9 coculture protocol provides enhanced. Human hematopoietic stem cells can survive in vitro for. Pdf mesenchymal stem cells mscs are multipotent stem cells capable of differentiating. Cell culture protocols thermo fisher scientific kr. In this study, we show not only op9 co culture, but factors secreted by op9 cells in isolation increase the proliferative potential of adult erythroid cells by. T cell culture and transduction the t cells are activated using aapcs, transduced with the carencoding viral vector, and expanded to large numbers in a bioreactor. Mammalian cell tissue culture techniques protocol abcam.
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