20.109(S11): TA notes for module 1: Difference between revisions

From OpenWetWare
Jump to navigationJump to search
Line 11: Line 11:


*Assuming about 3-4 groups don't have success at any given stage (hopefully more like 1-2), should have extra DNA fragments and RNA aptamers ready in time.
*Assuming about 3-4 groups don't have success at any given stage (hopefully more like 1-2), should have extra DNA fragments and RNA aptamers ready in time.
*etc
*Most important, have 1-2 extra tubes of purified RNA (both 6-5 and 8-12) ready for M1D4, diluted in Selection Buffer.


Scheme: each pair of students will prepare aptamer-encoding DNA, then each one (?) will do an IVT, and each will do her/his own column selection. Partners will do the same ratio of 6-5:8-12 and vary column washes, or perhaps vice-versa. (Maybe latter makes more sense for balanced use of materials?)
Scheme: each pair of students will prepare aptamer-encoding DNA, then each one (?) will do an IVT, and each will do her/his own column selection. Partners will do the same ratio of 6-5:8-12 and vary column washes, or perhaps vice-versa. (Maybe latter makes more sense for balanced use of materials?)

Revision as of 09:10, 23 June 2014


20.109(S11): Laboratory Fundamentals of Biological Engineering

Home        People        Schedule Spring 2011        Assignments        Lab Basics        OWW Basics       
RNA Engineering        System Engineering        Cell-Biomaterial Engineering              


General notes

S10 material all below; may need some revision (and Day 7 filling in looks like) for S11

Key preparation:

  • Assuming about 3-4 groups don't have success at any given stage (hopefully more like 1-2), should have extra DNA fragments and RNA aptamers ready in time.
  • Most important, have 1-2 extra tubes of purified RNA (both 6-5 and 8-12) ready for M1D4, diluted in Selection Buffer.

Scheme: each pair of students will prepare aptamer-encoding DNA, then each one (?) will do an IVT, and each will do her/his own column selection. Partners will do the same ratio of 6-5:8-12 and vary column washes, or perhaps vice-versa. (Maybe latter makes more sense for balanced use of materials?)

Day 1: Amplify aptamer-encoding DNA

Materials required:

The following could be up at the teaching bench in one ice bucket total, or could have one ice bucket shared per two bench spaces (4 total).

  • PCR Mastermix (from 5')
  • Forward and Reverse primers
    • Labeled "Forward Primer" and "Reverse Primer"
    • Original stock is 100 μM, intermediate is 20 μM
    • 3-4 tubes of enough 20 μM primer for 2-3 rxns each + 15% (each tube, not each pair)
  • DNA plasmid for aptamers 6-5 and 8-12.
    • 06.26.09 samples, original stocks are 2.48 and 2.68 μg/mL for 6-5, 8-12 respectively - ack! this was μg/μL - fixed before students made their samples
    • I have been adding ~ 2.5 ng by doing two sequential 1:100 dilutions, then adding 10 μL
    • For students' case, first dilute the plasmids 1:10, and let that be their original stock
    • Distribution scheme as for primers above

Day of Lab (R/F):

  • Thaw PCR Mastermix and mix well
  • Thaw and aliquot primers, diluted plasmid
  • Aliquot water to dilute plasmids

After Lab:

  • Freeze PCR samples when done.

Day 2: Purify aptamer-encoding DNA

Materials required:

On teaching bench unless otherwise noted.

  • DNA gel
    • 2:1 HR agarose gels ready on gel bench
      • ideally made a day in advance, or at least 3 hrs ahead, so they set thoroughly (cover w/plastic wrap to retain moisture)
      • Be sure to use thick side of comb.
      • Make sure to fully dissolve HR agarose in TAE and cook thoroughly (until clear)
      • Do NOT keep the gel in refrigerator overnight
    • Aliquots of 100 bp ladder (2-3 total) in orange freeze boxes on gel bench
    • Aliquots of loading dye - 1 per pair
  • On gel bench
    • Put up signs with sample table for reference.
    • Put out nitrile gloves.
  • DNA purification
    • Qiagen columns and buffers from kit
    • Aliquots of isopropanol
    • Aliquots of pH 7 water

Day of Lab (T/W):

  • Quiz (prepared by TA)
  • Thaw PCR products and DNA ladder shortly before lab.
  • Turn on water bath so it has plenty of warm-up time, e.g. when gels are started. Kept across from gel bench.
  • Test if all students have product after 30 min runtime; if missing product, run teaching aliquots for them on a fresh gel (30 min enough).
  • Collect and freeze purified DNA at the end of lab.

After Lab

  • Turn water bath back off.

How it went:

S11:

S10: W/F lab went substantially faster than T/R. Main difference seemed to be telling the students to weigh their eppendorfs for the gel slabs ahead of time, as well as warning about cutting small gel slices even more emphatically.

One group cut out multiple bands per lane, but their purified product looked fine when run on a gel (tested with 5 μL).

Running ~5-10uL of each group's leftover 6-5 and 8-12 DNA PCR fragments (3% HR Agarose gel + EtBr, 100V for 30 mins) showed that ALL Groups obtained bands of identical size and similar density. Thus, we expect that all groups should have successful IVTs if protocols were followed correctly.

Day 3: Prepare RNA by IVT

Materials required:

On teaching bench unless otherwise noted.

  • RNase free materials
    • Taped off area, bench paper, note about wearing gloves
    • Tip boxes, large and small
    • RNase away, kept in a box away from sunlight)
    • Eppendorf tubes
  • IVT
    • Aliquots of NTPs, T7, Ppase, KOH, pyrophosphatase (see google doc).
    • One per every 2 groups in their own ice bucket, enough for 5 rxns.

Day of Lab (R/F):

  • Quiz (prepared by TA)
  • Thaw their DNA shortly before lab.
  • Make sure 37 °C block is on.

After Lab:

  • After 4 hrs, RNA samples to -80 °C freezer

How it went:

S11:

S10: All groups on both days finished very quickly (indeed, today is an ideal day for long discussions such as Journal Clubs or writing workshops). Also, the IVT day also allows longer quizzes at the beginning of lab.

Day 4: Purify RNA and run affinity column

Materials required:

On teaching bench unless otherwise noted.

  • Equilibrate bead slurry in advance with SB.
    • Prepared each eppendorf individually instead of in a larger conical tube.
    • Not too far in advance though, as preservative will be diluted out.
    • e.g. 100μL beads per person in an eppendorf tube (total 2 per group); Add 200μL hemin beads and wash twice with 1X selection buffer.
    • Give beads in total 1mL volume to keep beads from sticking to sides of tube.
  • One 37 °C heat block, one 70 °C heat block ready.
  • Nutators up front. (Plus foil.)
  • RNase free materials available as on D3.
  • Extra ice bucket up front to collect RNA samples.
  • Lots of Selection Buffer!
    • Students use approximately 10mL per group (5mL per sample/aptamer-ratio); provide in a conical tubes.
    • Figure out in Google Doc.
  • Part 1
    • DNase aliquotted on ice, 1 per group, approx 20 μL.
    • Bring BioSpin columns out just ahead of time, or as needed (keep chilled)-- set on top of ice?
  • Part 2
    • Clean water, 3 mL per group to be safe.
    • 3 cuvettes per group.
    • Make sure students know to dilute RNA in SELECTION BUFFER and not water!
  • Part 3
    • Beads in SB (see above).
    • Per group, aliquot 200 μL of 125 μg/mL tRNA (1:100 of stock) and keep on ice.
      • Dilution in SB since students will be adding large quantities.
  • Part 4
    • Ring-stand with two grips per group.
    • Poly-prep columns and caps up front (1 per student).
    • Make fresh heme dilution to 2.5mM (from 11.1mM stock), each student/sample will need 200μL: aliquot ~450-500μL per group.
  • Part 5
    • Can be aliquotted or at least thawed during lab, not needed for a while. On ice.
    • Couple epps with 10-15 μL glycogen each-- to be shared among 2ish groups.
    • Few epps ammonium acetate, >=100 μL each.
    • One epp per group ethanol, 1.5 mL each.

Day of Lab (R/F):

  • Short quiz (prepared by TA)
  • Thaw student IVTs at last-minute, along with any reagents to be thawed.
  • Help students move through the lab in a timely fashion.
  • During the first half-hour, check their RNA calcs (hw) and flag any problems.

Days after Lab if relevant:

How it went:

Day 5: RNA to DNA by RT-PCR

Materials required:

  • HR gel (1 per day)
  • Aliquots of ethanol (room temp), 5 mL per group
  • Aliquots of 70% ethanol
  • Aliquots of RNase-free water, 110 μL per group
  • Ice bucket per 2 groups
  • Master Mix, 4 rxns + 15-20% per ice bucket (see google doc for recipe)
  • PCR tubes
  • Loading dye aliquots (minimum 10 μL per group, can share)

Day of Lab (T/W):

  • Quiz (prepared by TA)
  • When students get to the drying step...
    • Put out cold boxes
    • Check student samples to make sure they remove enough ethanol!!!
  • At the end, run and photograph gel with RT-PCR samples and ladder


Days after Lab if relevant:

How it went:

Day 6: Post-selection IVT and journal club

Materials required:

  • As Day 3, but half the amounts of everything.
    • S11: Gave the students a Mastermix of IVT materials to speed-up the prep so students could get to Journal Club.

Day of Lab (R/F):

  • Quiz (prepared by TA)
  • TA runs lab while Agi sets up journal club room

Day 7: Aptamer binding assay

Materials required:

  • Part 1
    • As Day 4 parts 1 and 2
  • Part 2
    • 6 μM heme stock, 1.2 mL per group
      • From ~ 1 M [presumably this should say 1 mM! -ANS] stock solution in DMSO
      • Dab a bit of solid into the solvent, then measure at 405 nm (extinction coefficient is 180 mM-1 cm-1)
    • 2x SB, 1.7 mL per group
  • Again, make sure students dilute RNA in selection buffer and not water!

Day of Lab (T/W):

  • Quiz (prepared by TA)
  • Turn on spec and the UV lamp partway through lab

Days after Lab if relevant:

How it went:

Day 8: Journal club

Materials required:

  • None - strictly a journal club day.
Retrieved from "https://openwetware.org/mediawiki/index.php?title=20.109(S11):_TA_notes_for_module_1&oldid=798408"