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RN46A大鼠永生化血清素能神经元细胞株NTCC® cell line BioVector NTCC质粒载体菌种细胞基因保藏中心

  • 价  格:¥599850
  • 货  号:RN46A
  • 产  地:北京
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BioVector® NTCC® RN46A大鼠永生化血清素能神经元细胞株NTCC® cell line

RN46a Cell Line
Cat No.: NTCC-012061302
Cell Line Origin
Embryonic rat medullary raphe, temperature-sensitive mutant of SV40 large T-antigen, immortalised, serotonergic, neuronal
Biological source
rat embryo (day 13 medullary raphe)
Growth mode
Adherent
morphology
Fibroblast morphology while proliferating and neuronal on differentiation
Cell Line Description
RN46A , an immortalized serotonergic neuronal cell line, was cloned by serial dilution following infection of dissociated embryonic
day 13 rat medullary raphe cells with a retrovirus encoding the temperature-sensitive mutant of SV40 large T-antigen (T-ag), RN46A
cells are capable of differentiating at 39 ° C the non-permissive temperature. Under differentiation conditions, RN46A cells cease
dividing, take on a neuronal morphology, and express enhanced levels of NSE and all three NF proteins. Differentiated RN46A cells
express low-affinity nerve growth factor (NGF) receptor (p75NGFR) and are i mMunoreactive using an antibody that recognizes the
carboxy-terminal 13 amino acids of all three trk proteins (pan-trk). Both i mMunoreactivities could be potentiated by treatment with
brain-derived neurotrophic factor (BDNF), NGF, and adrenocorticotropic hormone, fragment 4-10 (ACTH4-10). Differentiated RN46A
cells express low levels of tryptophan hydroxylase (TPH) i mMunoreactivity, which could be enhanced by treatment with ACTH4-10,
BDNF, or NGF. Low levels of serotonin i mMunoreactivity are detected in differentiated RN46A cells, and this was potentiated by
differentiating RN46A cells with BDNF for 8 d and 40 mM KCl for days 4-8. RN46A cells should prove useful to elucidate intracellular
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mechanisms that control neurofilament assembly and 5-HT expression in differentiating raphe neurons.
Culture Medium
DMEM:F12 (1:1) (D8062) + L-Glutamine (G7513) + 10% FBS / FCS (F2442) + 0.25mg/ml Geneticin (G418). Alternatively CNS
medium can be used (see Kawamoto & Barrett 1986). Differentiation can be induced as follows: cells growing at 33 ° C are subcultured
onto collagen/fibronectin matrix (100 μg/cm2 air-dried collagen I from rat tail followed by 1 μg/cm2 fibronectin). Subconfluent
cells (75%) are shifted to 39 ° C. The culture medium is changed to DMEM:F12 (1:1) (D8062) + 1%(w/v) bovine serum
albumin (BSA) + 1 μg/ml bovine transferrin + 5 μg/ml bovine insulin + 100 nM putrescine + 20 nM progesterone.
Subculture Routine
Split subconfluent cultures (70-80%) 1:2 to 1:5 using 0.25% trypsin/EDTA; 5% CO2; 33 ° C. Suggested seeding density 2-4 x 10,000
cells/cm2. Doubling time 19hrs.

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