DifferentiateEScellsintoglialcellsandneurons
Day -1: Pass ES cells at normal density on gelatinized plate to free the culture of contamination fibroblast cells.___________________Day 1: Trypsinized the cells as for normal passaging until the colonies lift off. Try to keep the loosely connected clumps of cells together by gentle handling. Then directly plate the cells 1:3 into bacterial grade Petri dishes in LIF free medium containing 1 microM all-trans ret......閱讀全文
Differentiate-ES-cells-into-glial-cells-and-neurons
Day -1: Pass ES cells at normal density on gelatinized plate to free the culture of contamination fibroblast cells.___________________Day 1:?Trypsiniz
Differentiating-Neural-Stem-Cells-into-Neurons-and-Glial-Cells
實驗概要The protocols in ?this section describe the steps involved in differentiating neural stem ?cells (NSC) to neurons, astrocytes, and oligodendrocyte
Differentiate-ES-cells-into-cardiac-myocytes
Day -1:?Pass ES cells at normal density on gelatinized plate to free the culture of contamination fibroblast cells.____________________Day 1:?Trypsini
Differentiate-ES-cells-into-cystic-embryoid-bodies
Day -1:?Pass ES cells at normal density on gelatinized plate to free the culture of contamination fibroblast cells.______________Day 1:?Trypsinized th
Differentiating-Glial-Precursor-Cells-into-Astrocytes-and-Oligodendrocytes
實驗概要Glial ?precursor cells (GPCs), also known as glial restricted progenitors ?(GRP) or oligodendrocyte progenitor cells (OPCs), are cells that have ?
KARYOTYPING-ES-CELLS
An actively growing culture of cells is required, i e 2 - 3 d ES cell culture. The total number of cells needs to be between 106 - 107 cells.N B Read
Electroporation-of-ES-cells
Cells are routinely passaged two days prior to electroporating. Usually one 10 cm plate at approximately 80% confluency will provide enough cells for
FACS-Analysis-of-ES-Cells
Isolate cells and dissociate to single cell suspension (can use Gibco Cell Dissociation Buffer, Accutase or Trypsin)Wash with 10% FBS/DMEM:F12For surf
Routine-Culturing-of-ES-Cells
Cell are normally passaged every 2-3 days, this is important to avoid differentiation.Signs of differentiation are:-i) colonies are surrounded by flat
Screen-ES-cells-by-Southern-Blot
Digest DNA in 96-well plateTo each well add:4ul 10Xbuffer4ul Enzyme0.4ul Spermidine(0.4M)31.6ul H2O37?C 19h, then add 4ul loading dye to each well. Lo
Derivation-of-Dopaminergic-Neurons-(from-Human-Embryonic-Stem-Cells)
實驗概要Directed ?differentiation of specific lineages has been a focal point in the ?field of human embryonic stem cell (hESC) research. Cell replacement
Human-Embryonic-Stem-(ES)-Cell-Protocols——Thawing-Human-ES-cells
Remove Human ES cells from liquid nitrogen storage tank. Fill out a freeze/thaw form.Thaw cryovial by gently swirling in waterbath until only a small
Human-Embryonic-Stem-(ES)-Cell-Protocols——Freezing-Human-ES-Cells
?Collagenase cells for approximately 7 minutes at 37 °C (until edges of colonies are curling up).With a 5 ml pipet, gently pipet and scrape colonies f
Human-Embryonic-Stem-(ES)-Cell-Protocols——Splitting-Human-ES-cells-on-MEFs
based on splitting onto one plateWarm collagenase IV split media to 37 °C in a water bath.Aspirate media off of cell culture plate.Add the following a
Human-Embryonic-Stem-(ES)-Cell-Protocols—Splitting-Human-ES-cells-onMatrige
based on splitting onto on plateWarm collagenase media to 37°C in a water bath.Aspirate media off of cell culture plate.Add the following amount of co
ELECTROPORATION-OF-ES-CELLS-AND-ISOLATION-OF-H/R-CLONES
Need 1.5-2 x 107 cells from a 2 day culture.1. Cells are harvested as normal, washed x 1 in PBS then taken up at conc. of 1.2 x 10 7 cells/ml in cold
胚胎干細胞和成體干細胞標志物
ContentsEmbryonic Stem Cell MarkersHematopoietic Stem Cell MarkersMesenchymal/Stromal Stem Cell MarkersNeural Stem Cell MarkersReferencesWhile stem ce
Primary-Cultures-fo...
實驗概要The following protocol provides a method of primary cultures for IHC – viability assays.實驗步驟1. Preparation of primary mesencephalic cultures??? 1)
Early-development-of-primary-motor-neurons-and-somites-in-Zebrafish-Embryos
Background:Zebrafish,or the teleost fish Danio rerio,is a rapidly developing organism that is apopular species for studying vertebrate development. Cl
二十碳五烯酸對大鼠海馬體突觸可塑性、不飽和脂肪酸...
二十碳五烯酸對大鼠海馬體突觸可塑性、不飽和脂肪酸綜合表現和磷酸肌醇3-激酶信號表達及對PC12細胞分化之影響安慰劑對照臨床研究表明, n-3多不飽和脂肪酸 (n-3 polyunsaturated fatty acids)能改善神經系統疾病 - 如阿爾茨海默氏病,亨廷頓氏癥和精神分裂癥等。為了評
Isolation,-Culture,-Characterization-of-Cortical-and-Hippocampal-Neurons
實驗概要The ?ability to culture primary neurons under serum-free conditions ?facilitates tighter control of neuronal studies. Some serum-free media ?and s
Culturing-Human-Neural-Stem-Cells
實驗概要Neural ?stem cells (NSC) are valuable resources because of their ability to ?differentiate into neurons and glial cells with applications in ?neur
Growing-feederindependent-embryonic-stem-cells§
We use feeder-independent ES cell lines derived from the 129/Ola strain of mice (Nichols et al., Development 110, p.1341, 1990). These cells are easy
Production-of-neuronpreferential-lentiviral-vectors
實驗概要Adenoviral vectors widely used to transfer foreign genes into neuronal cells possess tropism for glial cells and are toxic to infected cells.
Dissociated-Cultures-of-Cerebellar-Neurons
Dissociated Cultures of Cerebellar NeuronsHank Dudek (617-355-4735)Protocolisolate cerebella (òCbó)cut off head into plate with HHGNhold nose with lar
stem-cell-culture-protocol
實驗概要stem cell culture protocol主要試劑cell culture supplies and reagentssEnvironment: cell culture requires a sterile environment, so it needs a separat
Derivation-and-Culture-of-Dopaminergic-Neurons-(from-Midbrains-of-Rodents)
實驗概要Dopaminergic ?(DA) neurons are located in the ventral midbrain (VM). The ability to ?isolate precursor cells and neurons from the VM provides a po
ES-Cell-Culture-and-Manipulation2
Picking ES cell clonesOne or two days before picking colonies prepare 24-well plates of feeders. You can also use alternate protocols that utilize 96-
Detection-of-MicroRNA-Heterogeneity-in-Single-Cells-Using-an-Automated
Introduction ?MicroRNA ?(miRNAs) are short (18–24 nucleotides), non-coding RNAs that regulate ?gene expression by both disrupting messenger RNA (mRNA
自動化的微流控芯片系統在單細胞中檢測MicroRNA的異質性3
結論·? 我們在C1TM單細胞自動制備系統開發了一種簡潔的實驗方案,能以最少的手工操作,在不到24小時內,平行處理高達96個單細胞,對其miRNA表達譜進行分析。·? C1 miRNA STA實驗方案使用了Life Technologies為miRNA優化過的試劑。特別的,Megaplex? RT及