Hi everyone, gwen here. I am going to share with you about MTT assay. This assay is done to determine the potency of the drug and proteins used for cancer therapy. Each treatment can consist of the drug with the protein or just the drug or protein alone.
The first step to this assay would be to seed the desired cells into 96-well plates. The number of plates needed would depend on the number of treatments planned. The cells would then be incubated and treated with treatments the next day. Each plate will have 12 columns altogether. 2 columns are reserved as controls and the cells in the remaining 10 columns of cells will be treated with the treatments.
After overnight incubation, the MTT (3-(4,5-Dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide, a tetrazole) solution is added to the cells after removing the used media/treatments. The plates are then incubated for another 3-5 hours. During this time, the MTT forms purple formazan from the living cells. After the incubation, the remaining MTT solution would be removed. Care must be taken so as not to pipette the purple formazan out, as it will affect the viability results.DMSO is then added to each well of the plate so as to dissolve the purple formazon, then the absorbance level can be read and the viability of the cells determined. Viability is calculated by dividing the absorbance level of the treated cells with that of the control and a percentage is derived.
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Hi gwen! :D
ReplyDeleteI would like to ask what is the purpose of adding the MTT solution?
Also, why must the purple formazan be pipetted out for absorbance reading?
Thanks in advance!
(:
Siew Ming
0702862D
TG 01 Grp 2
HI Siew Ming!
ReplyDeleteThe MTT solution is added to form the purple formazan from the cells. TO read the absorbance levels, the purple formazan must be dissolved in DMSO. Thus the MTT solution must be removed as it would affect the absorbance levels. Hope this answers your question. Thank You :)
Gwendolynn Tan
0703953J
TG02
Gwen gwen gwen!!!
ReplyDeletei have a qn for u..
what is purple formazan? How is it related to the cells?
Zhang'e
0704086H
TG02
hi gwen!
ReplyDeletei've actually realised i forgotten to ask this in stanley's post, but since both is about MTT, so i'll ask here.
so is there a need to remove media, and how will the MTT solution affect the absorbance? as i am doing MTT assay also, i've actually checked out several websites, and they argued what's the difference between removing and not removing the solution. therefore i'm confused.
(:
lim jia hui
tg01 0703605F group 2
Hi
ReplyDeleteIs it necessary to dilute the purple formazan in DMSO? Are there any alternative diluents to consider, eg: deionized water?
Liyana
0703827F
Gwen,
ReplyDeleteRemoval of media - what if you remove the cells together too? What do you do?
Li Yinliang Alex 0704894E
TG02 Group 8
8 September 2009
HI ALL!!
ReplyDeleteReally sorry for the late reply...
Zhang'e: The purple formazan is a crystal that is formed when the the MTT is reduced to form purple formazan in living cells. As this assay is to determine viability of the cancer cells after treatment, we must thus know the amount of living cells.
Joey: Towards this dispute, i am also not too sure what is the difference. I asked mt mentor about it but she said that the reason was too unknown to her. I have also tried seraching it in the net but to no avail.
Liyana: Yes it is neccessary to dilute the purple formazan as we are measuring its absorbance level. There are definitely other diluents to consider but DMSO is the least harmful and not volatile so we will not inhale the vapours. DI water is not used as the purple formazan are not soluble in it.
Alex: The cells are attached to the base of the well so the chances of removing the cells while sucking up the media is highly unlikely unless the cells is semi adherent as in the case of a cetain cancer cell line, SH-SY-5Y. In this case, removal of medium will have to be done slowly. But if the cells were really sucked up, we would not know until examination under the microscope. The most important thing when removing media is also not to scratch or poke the base of the well with the pipeete tip.
Thank you for asking me questions. I hope that i have answered your questions:) Once again sorry for the late reply.
Cheers,
Gwendolynn Tan
0709953J
TG02
sir i have done this method twicly with mice spleen lymhpocytes as 25000cells/well but no absorbence observe could u explain me what is the reason behind it?
ReplyDelete