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運(yùn)輸方式：凍存運(yùn)輸
ATCC Number：ACS-1004?
相關(guān)疾?。浩渌膊?br /> 年限：16 years
數(shù)量：大量
細(xì)胞類型：其他細(xì)胞類型
是否是腫瘤細(xì)胞：0
物種來(lái)源：人
規(guī)格：0.5mg                                                                                                                                                                                                                                                                                                                                                          Designations: ATCC -DYP0250 Human Induced          Pluripotent Stem Cells
         Depositors:                  ?ATCC
         Biosafety Level:2 [ATCC highly recommends that            protective gloves and clothing always be used and a full            face mask always be worn when handling frozen vials.          It is important to note that some vials leak when submersed            in liquid nitrogen and will slowly fill with liquid            nitrogen.  Upon thawing, the conversion of the liquid            nitrogen back to its gas phase may result in the vessel            exploding or blowing off its cap with dangerous force            creating flying debris.  ]
         Shipped:        frozen
         Medium & Serum: See Propagation                    Organism:          Homo sapiens
         Morphology:          

         Source:          Disease:  Cystic fibrosis
         Cell Type:  Human iPSC
         Reprogramming Method:  Episomal expression of            OCT4, SOX2, KLF4,  and MYC  genes
         Permits/Forms:In addition to the MTA          mentioned above, other ATCC            and/or regulatory permits  may be required for the          transfer of this ATCC material. Anyone purchasing ATCC          material is ultimately responsible for obtaining the permits.          Please click here  for information regarding          the specific requirements for shipment to your location.
             Restrictions:This product may be used by          investigator for internal research purposes and only in          recipient's investigator's laboratory subject to the iPS MTA,          the Addendum to the iPS MTA, and any additional third party          terms. This product is subject to claims under U.S. Patent          Nos. 8,058,065 and 8,048,999, pending patent applications, and          foreign counterparts thereof.  For information on obtaining          additional rights, please contact licensing@ATCC .org          .The iPS MTA and Addendum to the iPS MTA are also available          at: www.atcc.org .
         Age:        16 years
         Gender:        Male
         Ethnicity:        Unknown
         Propagation:                   ATCC complete growth medium:  CellMatrix?          Basement Membrane Gel                                
         CellMatrix? Basement Membrane Gel          
Pluripotent Stem Cell SFM XF/FF
Pluripotent Stem          Cell SFM XF/FF

         Subculturing:        This protocol is designed to passage          stem cell colonies cultured in a 6 cm dish, using Stem Cell          Dissociation Reagent (ATCC ACS-3010 ) to detach the cell colonies.          Stem Cell Dissociation Reagent is stored as a 0.5 U/mL working          solution at -20°C. The cells should be split at a ratio of          1:4.
Volumes should be adjusted according to the size          and number of the tissue culture vessels to be          processed.
1.  Warm an aliquot of Stem Cell Dissociation          Reagent working solution to room temperature.
2.          Aspirate and discard the stem cell culture medium.
3.          Rinse the cells twice with 4 mL of D-PBS (ATCC 30-2200 ).
4.  Add 2 mL of Stem Cell          Dissociation Reagent working solution to the dish.
5.          Incubate at 37°C for 10 to 15 minutes or until the edges of          the individual colonies begin to loosen and fold back. View          the dish under the microscope starting at 5 minutes as          incubation time will vary depending on the cell line and          colony size.
6.  Aspirate the Stem Cell Dissociation          Reagent and gently rinse the colonies with 4 mL of DMEM: F-12          Medium (ATCC 30-2006 ), taking care not to dislodge the          cells during manipulation.
7.  Add 2 mL of Pluripotent          Stem Cell SFM XF/FF to the dish, and detach the cells by          pipetting up and down several times with a 1 mL tip. Take care          not to over-pipette the culture into a single-cell suspension          as single cells will not establish colonies after          seeding.
8.  Transfer the cell aggregates to a 15 mL          conical tube.
9. Add an additional 3 mL of Pluripotent          Stem Cell SFM XF/FF to the dish to collect any remaining          cells. Transfer this rinse to the 15 mL conical tube          containing the cell aggregates.
10. Centrifuge the cell          aggregates at 200 x g for 5 minutes.
11.  Aspirate the          supernatant and discard.
12.  Gently resuspend the          pellet by pipetting up and down 5 to 6 times with a 1 mL tip,          maintaining the small cell aggregates.
13.  Plate the          cells as desired on feeder or feeder-free cultures in the          presence of 10 ?M ROCK Inhibitor Y27632* (ATCC ACS-3030 ) to the cell culture medium is          recommended.
*ROCK Inhibitor Y27632 has been shown to          reduce dissociation-induced apoptosis.
14. Incubate the          culture at 37°C in a humidified 5% CO₂ /95% air          incubator. Perform a 100% medium change every day. Passage the          cells every 4 to 5 days (80% confluent).
         Preservation:        For optimal results, cryopreserve stem          cell colonies when the cell cultures are 80% confluent. This          protocol is designed to cryopreserve stem cell colonies          cultured in a 6 cm dish.
1.  Detach stem cell colonies          from the dish as described in the recommended subculturing          protocol (steps 1-11). Gently tap the bottom of the tube to          loosen the cell pellet.
2.  Take the Stem Cell Freezing          Medium (ATCC ACS-3020 ) from storage and swirl to mix.          Keep cold. Decontaminate by dipping in or spraying with 70%          alcohol.
3.  Add 2 mL of cold Stem Cell Freezing Medium          to the tube. Gently resuspend the pellet by pipetting up and          down 5-6 times with a 1 mL tip, maintaining the cell          aggregates.
4.  Immediately transfer 1 mL each of the          cell suspension into two labeled cryovials.
5.  Freeze          the cells gradually at a rate of -1°C/min until the          temperature reaches -70°C to -80°C. An isopropanol freezing          container also may be used.
6.  The cells should not be          left at -80°C for more than 24 to 48 hours. Once at -80°C,          frozen cryovials should be transferred to the vapor phase of          liquid nitrogen for long-term storage.
         Related        Products:Stem Cell Dissociation Reagent (ATCC          ACS-3010)
D-PBS (ATCC 30-2200)
ROCK Inhibitor          Y27632 (ATCC ACS-3030)
DMEM: F12 (ATCC 30-2006)
         Stem Cell Freezing Media (ATCC ACS-3020)