Eukaryote Growth Dynamics

互联网2013-09-05

606

LEVEL II

Materials

Suspension cultures set up from Exercise 12.8

Sterile transfer pipettes

Materials for viability counting ( Exercise 12.7 )

Procedure

1. After 12 hours, aseptically remove 0.1 ml from each of the three cultures, add 0.1 ml of trypan blue and count the total number of cells and the number of blue cells. Compute the number of viable cells/ml.
2. After 24 hours (from the time of seeding), repeat step 1.
3. Continue to repeat step 1 at 24 hour periods (i.e. daily) until there is no change in the number of cells/ml of culture.
4. Plot cell concentration on a log scale vs time of culture. Identify and label the Lag, Log and Plateau phases for your culture.
5. Select a period of time during the Log Phase and compute the doubling time for your culture. That is, the time required during the Log Phase to exactly double the number of cells/ml.

相关产品推荐

thermo特约代理商|A15026 RiboMinus™ Eukaryote System v2

￥3000

EGFR/EGFR蛋白Recombinant Human Epidermal growth factor receptor (EGFR) (Active)重组蛋白Proto-oncogene c-ErbB-1 (Receptor tyrosine-protein kinase erbB-1 ) (ERBB) (ERBB1) (HER1)蛋白

￥1368

RMDN3/RMDN3蛋白Recombinant Human Regulator of microtubule dynamics protein 3 (RMDN3)重组蛋白Cerebral protein 10Protein FAM82A2;Protein FAM82;CProtein tyrosine phosphatase-interacting protein 51TCPTP-interacting protein 51蛋白

￥1344

TrEMBL/TrEMBL蛋白Recombinant Sus scrofa Platelet-derived growth factor subunit B重组蛋白/蛋白

￥1836

IGF1/IGF1蛋白Recombinant Chicken Insulin-like growth factor I (IGF1)重组蛋白IGF-I;Somatomedin蛋白

￥1656