Anyway, for your information, i am currently working at a Oncology (cancer) research institute and everyone in my group is actually pretty much working on their own projects though we have general lab meetings every alternate weeks to update each other on our research progress etc etc.
As for me, i am focusing on a particular gene (let's just call it gene A) to see if there is an over-expression of it in prostate cancer. If there is a huge amount of gene A found in the prostate cancer cells, we can then make assumptions that perhaps this gene A has something to do with encouraging tumour angiogenesis or cancer cell proliferation etc etc. From it, we will then be able to find out if we could come up with an inhibitor that can block the action of the proteins (translated from gene A) and hopefully treat this cancer! (ok, this is the simplified version of my job scope. it's so much more complicated if i really want to elaborate but i will just leave it as that ok? =] )
For the past 3 weeks, i have been trained on Immunohistochemistry (IHC) which is very commonly used in cancer research to allow one to check if a particular protein is present/over-expressed in the cancer cells of that particular organ of the body. If you can still recall what we learnt during HistTech, it's 90% exactly the same as the staining we did =)
IHC: Materials and Methodology
1) As tissue samples from hospitals normally are formalin-fixed/paraffin-embedded sections, deparaffinization was done in 3 consecuetive xylene baths for 5 mins each
2) The slide was then dipped into 2 changes of absolute alcohol for 5 mins each as well.
Significance: To remove xylene from the slides and to prepare the sections for rehydration. This is because xylene and water are NOT miscible.
3) Rehydration was then performed as the slide was dipped in 95% alcohol (2 changes, 5mins each) before it was placed in 75% alcohol (2 changes, 5mins each). Rehydration is considered complete when the slide was rinsed with tapwater.
4) Pre-treatment was carried out as the slide was immersed in Ag Retrieval Buffer before it was placed in the Mega Microwave Histoprocessor at 117 degree Celsius for 30 mins.
Significance: When you fix a tissue sample using formalin, what it does is to denature proteins by coagulation, by forming additive compounds or by a combination of the 2. As a result, confomational changes in the protein structures will then occur to inactivate the enzymes and preserve the cells/tissues. Therefore, this pre-treatment process is to "revive" the immunoreactivity of the Ag to an immunogen. This process is aka "epitope retrieval" process.
5) The slide was cooled for 20mins before it was dripped dry and encircled using a Dako Pen
Significance: Dako pen is able to "trap" whatever reagents used on the sample within the encircled area so we don't have to use too much reagents and waste them.
6) Peroxidase block was added for 10 mins to the section to block any endogenous peroxidase that was produced by the cells.
Significance: Our secondary Ab will be labelled with Horseradish Peroxidase. Hence, we don't want any false positive results because of the presence of endogenous peroxidase.
7) Slide was washed to remove any excess peroxidase block reagent.
8) Ready-to-use Protein Block was used on the slide for 1 hour
Significance: Remember we have learnt about the "blocking" step in MBio last semester? It works in the same theory: to prevent non-specific binding.
DO NOT WASH SLIDE THIS TIME ROUND because even if you feel that the protein block might block the antigens in which the primary Ab have to bind to, this is not true. According to my senior, as the primary Ab used is more specific to the Ag than the protein block, it will have a higher affinity and the former can eventually replace the protein block. Hence, the end results will not be affected.
9) Primary Ab was then added to the slide for 1 hour. For every different kind of Ab used, we have a specific dilution for it. In case you are curious to know, i am using 1:5000 dilution =)
10) Washing was done this time to remove excess Ab
11) Secondary Ab labelled with HRP was added. Since my primary Ab is raised in mouse, my secondary Ab is an anti-mouse solution yup!
12) Washing carried out again
13) Chromogen and DAB was then added for just 5 minutes.
Significance: DAB will oxidise when it comes into contact with the air in the environment causing polymerisation and increasing its staining intensity. Chromogen is the substrate that will bind to the HRP to give us the signal we want.
14) After the slide was rinsed with tap water, it was counterstained using only Mayer's Haematoxylin.
Significance: As recent research has shown that protein A (from gene A) will be localised only in the nucleus, we only have to use haematoxylin and can save on our Eosin dye.
15) Dehydration was then carried out as the slide was dipped into 75% alcohol (2 changes, 5 mins each), 95% alcohol (2 changes, 5 mins each) and lastly absolute alcohol (2 changes, 5 mins each)
16) The slide was placed in the fume hood for 10 mins for drying to completely remove any water present on the slide/sample
Significance: water and xylene = NOT miscible
17) Lastly, the slide was placed in xylene for 3 changes for 5 mins each before it's mounted using DPX
Example:
Figure 1. Prostate cancer tumour sample expressing gene Z (Nucleus gives dark brown coloration). Note that only Mayer's Haematoxylin was used because researchers already know that gene Z staining is mainly localised in the nucleus.
Image is taken with permission from fellow co-worker.
Hope i didnt get my concepts wrong. LOL. correct me if you think i am inaccurate in any way yup =) Anyway, hope you guys are enjoying SIP over at your side.
Psst: should u have too much time to spare, u can join me for lunch coz i m alone like nisha as well! haha.
KangTing TG02
0503331A
19 comments:
hey kangting!
your attachment sound interesting..heex.
now is the question time.. u mentioned the use of dako pen ? any other alternatives besides using this and how does it helps in "trapping" reagents?
kai lin =)
to KAILIN:
hello! Hmmm. All my colleagues use Dako Pen because it's actually "water-repelling". Which is why when u draw a circle around ur sections right, this circle will act as a barrier to prevent any liquid (like my pri. Ab) from flowing OUT of the circle =)
Erm...i dun think there are any alternatives at the moment..but DAKO is the brand's name! So meaning there is the possibility that other brands have very similar products too =)
hihi kangting,
yours SIP sound interesting. :)
i have a question. u mention about DAB, what does it stand for? and you mention about there is specfic dilution for the Ab. what is the purpose of the dilution?
Juexiu
tg02
to JUE XIU
Hellooo. i knew someone is gona ask abt DAB!!! haha. let me go back to my lab on Mon and check out the full name for u k? =)
As for dilution, think abt it, if my dilution for my primary Ab is like 1:5000. However, i decided to put 1:100 of dilution instead. What will happen? the Ab will most probably bind to the other Ag that are NOT SPECIFIC to it at all because it is in such high concentrations. Hence, after staining, the whole slide will become brown in color, giving false positive results =)
hello kangting,
U said that u used different Ab right? Why and when u know that u need to use which type of Ab? Thanks ya!
Michelle
to MICHELLE:
oh, to verify different Ag (on diff proteins), we must use different Ab right? For example, Ag A on a protein will require a specific Ab to bind to it, in this case, Ab A! Get it?
kangting!
the blocking agent can be washed off easily?so am i rite to say that if the blocking agent binds to the Ag, the Ab is able to like snatch the blocking agent's place?
and yah, ur blog is detailed! haha..have fun gal!
charmaine
TG01
hey! today i just found out got this hill behind cels. so cool, like another world. You shd go see it sometime.
Anyways, must the Haematoxylin be Mayer's Haematoxylin or can other types of Haematoxylin be used? Whats so special about mayer's from the other types of haematoxylin?
- Debra, tG02
to CHARMAINE:
hey girl! How's ur in-house??
Yup! That is correct, at least that was what was explained to me by my senior =) He said it's because as compared to the blocking agent, the Ab is MORE SPECIFIC to the Ag.
To JUE XIU (agn. haha.) :
DAB stands for Diaminobenzidine =)
to DEBRA:
ANOTHER HILL! omg. okok. i go check out soon =)
Anyway, i realised another alternative for Mayer's Haematoxylin is Gil No.3 but i don't know why they are chosen for staining. If i find the answer, will let u know k!
Hi kangting!
You mentioned about the Ready-to-use Protein Block. What is it made up of? Coz previously in MBio, we know its milk proteins right?
Cool man, your SIP. i'm almost jealous. hehehe.
Sharifah
TG01
to SHARIFAH:
oooh, for me, i am using Goat Serum as my protein block because my secondary Ab is raised in goat. =) If not, i think BSA solution is fine too! Er..should be 3-5% BSA solution. hee. I think the milk proteins thing is used in the Western Blot? not IHC.
Ohhh, wait till u listen to my stories then u will not be jealous anymore. LOL.
Hi
After you add the primary or secondary antiobody to the (antigen)slide, you have to incubate for a certain amount of time right?
I just wanna know at what temperature do you incubate the slide (room temp: or 37C)or is there any requirement in the incubation, e.g. moist chamber?
~Ye Tun
TG01
Hi kangting!
You stated that pre-treatment is needed to 'revive' the reactivity. So will the test be greatly affected if pre-treatment step was not carried out?
Thank you for your time! Take care!
Yvonne Lau
TG01
To Ye Tun:
Hello! Yup..different Ab will lead to different incubation time. In my case, the temp i use is simply room temperature in slightly moist environment. However, in any case shld u need to incubate the primary Ab overnight, my senior always does it at 4Degree Celsius =)
To Yvonne:
hi! Yup, it wld definitely GREATLY AFFECT the entire staining process because in this way, the immunoreactivity of the Ag cannot be revived and it cannot bind to the primary Ab and sec Ab and lead to very poor staining results.
hi kangting
your SIP sounds very interesting. Anyway you mentioned something about "DO NOT WASH SLIDE THIS TIME ROUND" i dont really quite understand this part? don mind can u explain to me on this part again??
Vinodhini
TGO2
To Vino:
Oh, if u realise, after adding all the primary Ab etcetc, i will say slides will be washed to remove any unbound/excess reagent. However, in this case, after adding the protein block, washing is not done because u might remove the block that can help prevent non-specific binding from occurring.
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