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Effects of Sheep Brain-Derived Factors on Primary Cultures of Kidney Cells

Effects of Sheep Brain-Derived Factors on Primary Cultures of Kidney Cells. Authors: Mohammed Yahia Ismaiel Alswalhe, Mohammad Yousef Manaserah , Hasan Altarda and Dr Robin Abu Ghazaleh. Introduction.

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Effects of Sheep Brain-Derived Factors on Primary Cultures of Kidney Cells

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  1. Effects of Sheep Brain-Derived Factors on Primary Cultures of Kidney Cells Authors: Mohammed Yahia Ismaiel Alswalhe, Mohammad YousefManaserah, HasanAltarda and Dr Robin Abu Ghazaleh

  2. Introduction • Sheep and rabbit organs were collected and assessed for growth properties at the PPU Biotechnology Research Center’s (BRC) animal cell culture unit. • The growth characteristics of adult tissues were too slow to be practicably viable, but new-born organs generated cells capable of rapid growth.

  3. Introduction • New growth factor was applied in PRC that is derived from the brain of sheep. • The standard protocol that use a delicate mix of exogenous growth factors that are very costly to purchase. • This G.F have the ability to supplement the growth of primary cell cultures at a fraction of the cost of using commercially available cell lines of growth factors for primary cultures.

  4. Introduction • The pig brain-derived factors have the mitogenic enhancing effect. • sheep brain would give a species-specific advantage.

  5. Objective • To determine optimal growth condition of primary cells which is necessary requirement for in-vitro testing of anti-cancer drugs, vaccines and infectious diseases of livestock.

  6. Cell culture methodology

  7. Cell culture result Figure 2. Growth curves for sheep kidney cells cultured in DMEM medium with various quantities of brain extracts in ml. Error bars are standard deviations, and n = 5 replicates.

  8. Cell culture result (b) (a) 0.5 1.0 0.0 Sheep brain extract supplementation, ml. Sheep brain extract supplementation, ml. Figure 3. Effect of xeno-supplementation upon proliferation of rabbit kidney cells with sheep brain extract in (a) DMEM for 7 days and in (b) RPMI medium for 4 days. Error bars are standard deviations, and n=10 replicates were performed for the zero supplement controls and n=5 for the supplementation with sheep brain extracts.

  9. Cell culture result Figure 4. Senescence curve for rabbit lung cells in RPMI without supplementation. Error bars are standard deviations, and n = 5 replicates.

  10. Cell culture result (b) (a) (a) (b) Figure 1. Confluent kidney cell monolayer at 100X magnification through a phase contrast inverted light microscope.

  11. Conclusions • Healthy monolayers of sheep kidney cells can be cultured using new born sheep kidneys with DMEM medium and supplementation with brain extracts. • Input of higher quantities of brain extract had an inhibitory effect, indicating the presence of competing enhancing and inhibitory factors that interact depending upon different dosage rules to give an overall enhancement in growth rate at lower quantities and an overall inhibition at higher quantities.

  12. Conclusion • Use of the sheep brain extract for xeno-supplementation confirmed that the growth enhancing effects were species-specific while the inhibitory effects may be non-specific in nature.

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