http://bmcwiki.mit.edu/index.php?action=history&feed=atom&title=BioMicroCenter%3AClusteringBioMicroCenter:Clustering - Revision history2026-04-29T03:18:35ZRevision history for this page on the wikiMediaWiki 1.43.1http://bmcwiki.mit.edu/index.php?title=BioMicroCenter:Clustering&diff=36&oldid=previmported>Allison Perrotta at 21:54, 28 January 20092009-01-28T21:54:46Z<p></p>
<p><b>New page</b></p><div>{{BioMicroCenter}}<br />
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Preparing Reagents for the Cluster Station <br />
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Denaturing and preparing samples: <br />
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*Label two rows of 1.5mL microcentrifuge tubes 1 through 8, one for denaturation and one for final dilution (this one is the pre-chilled hyb buffer) <br />
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*Dilute samples to 10nM using Illumina Dilution excel worksheet (do this into 1st row of labeled tubes, don’t need to dilute Phix) <br />
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*Aliquot 996uL of Hybridization buffer into 8 1.5mL microcentrifuge tubes (2nd row of labeled tubes) place these on ice (amount of Hybridization buffer will change if doing over 4pM)<br />
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*Make master mix of EB and 2 N NaOh, 162uL EB + 9uL NaOH (total of 171uL) vortex and spin (the amount of EB will change if doing over 4pM)<br />
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*Aliquot 19uL of EB/NaOH master mix into 8 1.5mL microcentrifuge tubes (2nd row of labeled tubes). Then add 1uL of each sample (including Phix). These amounts will change if doing over 4pM. Vortex, spin, and place on ice.<br />
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*Add 4uL of each denatured sample to the tubes containing the pre-chilled Hybridization buffer (this amount will change if doing over 4pM). Vortex and spin. Keep these tubes on ice until you are ready to load stip B onto the cluster station. <br />
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*Take out -20 cluster box. Take everything out. Put the enzymes and nucleotides on ice and leave TE and cluster buff out on the bench to defrost. <br />
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*Start making the Amp, Lin, Block reagents:<br />
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Label 6 50mL tubes Reagents #1, #9, #10, #11, #12, and Amplification Pre-mix<br />
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Label two 15mL tubes Reagent #3 and Blocking Buffer1X<br />
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Label three 1.5mL screw caps Reagent #5, #14, and #15<br />
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Also label a 1.5mL microcentrifuge tube "E"<br />
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- Reagent #3 (Linearization buffer):<br />
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o Add 1518uL (or 759uL x 2) of dH2O to the tube of Sodium Periodate<br />
o Vortex until dissolved<br />
o In a 15mL conical tube, add 60uL 1.0 M Tris to 1500uL formamide<br />
o Mix thoroughly<br />
o Transfer 1437uL (or 718.5uL x 2) of the sodium perodate solution into the 15mL conical tube of formamide/tris solution. <br />
o Mix thoroughly.<br />
o Add 2.3uL of 3APL to the solution in the 15mL conical tube (NOTE: 3APL is a viscous solution. Wipe and excess from the outside of the tip before adding it.)<br />
o Mix thoroughly<br />
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o Set aside until you are ready to load the reagents on the cluster station.<br />
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- Reagent #15 (Blocking Buffer 1X): <br />
o Dilute 300uL Blocking buffer 1 to 1x concentration with 2700uL deionized water<br />
o Transfer 1400uL of the 1x blocking buffer into a 1.5mL screw-cap tube<br />
o Set aside until ready to load reagents on the cluster station<br />
- Reagent #5 (Blocking Mix): <br />
o Prepare the blocking mix by mixing the following on ice:<br />
1510.2uL (or 755.1uL x 2) of Blocking Buffer 1X<br />
30.1uL of 130uM ddNTPs <br />
19.7uL of Terminal Transferase <br />
the total volume is 1560uL<br />
o Set aside on ice until ready to load it onto the cluster station<br />
- Reagent #9 (Formamide):<br />
o Transfer 15mL of formamide into the tube<br />
- Reagent #10 (Wash buffer)<br />
o Transfer 10mL of wash buffer into the tube<br />
- Reagent #12 (Storage buffer)<br />
o Transfer 5mL of storage buffer into the tube <br />
- Reagent #14 (Deionized Water) <br />
o Transfer 1.5mL into the tube<br />
- Reagent #11 (Amplification Pre-Mix)<br />
o To prepare this mix the following into a 50mL tube: <br />
15mL Water<br />
3mL Cluster buffer<br />
12mL Betaine 5M<br />
The total volume should be 30mL<br />
o If the room temp is high this mix might be cloudy, you can put it on ice to avoid this<br />
o Filter this mix with a 0.2um cellulose acetate syringe filter. <br />
o Transfer 12mL of the Amplification mix to the 50mL tune labeled #11 and leave the rest for use in other reagents.<br />
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- Tube Strip E (initial extension mix)<br />
o Initial extension mix using Taq polymerase:<br />
o Prepare this mix by mixing the following on ice in a 1.5mL epindorph tube:<br />
975uL of Amplificatn pre-mix<br />
20uL of 10mM dNTPs<br />
5uL of Taq DNA polymerase<br />
The total volume should be 1000uL<br />
o Place this on ice until tube strip D is on the cluster station<br />
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- Reagent #1 (Amplification mix with Bst DNA Polymerase)<br />
o Mix the following in the 50mL tube: <br />
12mL Amplification Pre mix<br />
240uL of 10mM dNTPs<br />
120uL of Bst DNA Polymerase<br />
The total volume should be 12.36mL<br />
o Set this tube aside on ice until you are ready to load it on the cluster station<br />
- Tube Strip A:<br />
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o Aliquot 140uL pf Hybridization buffer into each tube of a tube strip<br />
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- Tube Strip B:<br />
o Strip B is 120uL of each sample in the tubes of a tube strip (don’t do this until strip A is on the cluster station)<br />
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- Tube Strip C:<br />
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o Aliquot 100uL of wash buffer into each tube of a tube strip (don’t do this until B is on the cluster station<br />
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- Tube Strip D: <br />
o Add 100uL of the amplification mix into each tube of a tube strip, don’t do this until C is on the cluster station<br />
- Tube Strip E: <br />
o Use initial extension mix made above, on ice, aliquot 120uL into each tube, don’t do this until D is on the cluster station.</div>imported>Allison Perrotta