Inoculated 5mL of 1xLB + Kan50 with re-streaked colonies from 20110707. Incubated O/N, 37C, 200RPM. Will isolated plasmids of those with inserts tomorrow.
Tag Archives: prostaglandin synthase
Clone Restreaking – PGS2 Hi/Lo Clones (from 20110421)
Sequencing of the PGS2/COX2 clone failed (was empty vector). Restreaked bacterial clones on to a Kan50 plate (made 20110413 by SJW) from a plate that Caroline Storer had created from cloning colony selection on 20110421. Samples were labeled as PGS Lo 1 & 2 and PGS Hi 3 & 4. Additionally, there were red numbers on the plate associated with these four samples. They were 42 – 45, respectively. PGS Hi 4 (#45) was previously grown up and sequenced. This sample is what produced vector only sequence. Incubated O/N @ 37C. Hopefully we’ll bacteria is still viable and will have samples to grow up for miniprep, plamsid iso and sequencing.
Results:
Limited growth in all after O/N incubation. Will leave plate on bench over the weekend and hope to get more growth.
After the weekend on the bench, have growth in all but PGS Lo 2. Will inoculate liquid cultures for plasmid preps.
qPCR – C.gigas COX2 on V.vulnificus exposure cDNA (from 20110311)
Ran a qPCR on all cDNA samples from the V.vulnificus exposure experiment from 20110111. Primers used were Cg_COX1/2_qPCR_F (SR ID: 1192) & Cg_COX2_454align1_R (SR ID: 1190). Samples were run in duplicate. Master mix calcs are here. The master mix info is the same that was used earlier today, but with the primers noted above, not those listed on the calcs page. Plate layout, cycling params, etc., can be seen in the qPCR Report (see Results).
Results:
qPCR Data File (BioRad CFX96)
qPCR Report (PDF)
Data looks good (e.g. the replicates are all very close, with the largest Cq Std. Deviation = 1.227, although this does appear to be an anomaly as the next highest Cq Std. Deviation in any of the reps is 0.633), nothing in the NTCs, & the melt curves look good. Will eventually normalize the data and then perform a complete analysis.
qPCR – C.gigas COX1 on V.vulnificus exposure cDNA (from 20110311)
Ran a qPCR on all cDNA samples from the V.vulnificus exposure experiment from 20110111. Primers used were Cg_COX1/2_qPCR_F (SR ID: 1192) & Cg_COX1_qPCR_R (SR ID: 1191). Samples were run in duplicate. Master mix calcs are here. Plate layout, cycling params, etc., can be seen in the qPCR Report (see Results).
Results:
qPCR Data File (BioRad CFX96)
qPCR Report (PDF)
Data looks good (e.g. the replicates are all very close, with the largest Cq Std. Deviation = 0.534), nothing in the NTCs, & the melt curves look good. Will eventually normalize the data and then perform a complete analysis.
Bacterial Cultures – Colonies Selected from Yesterday’s Colony PCRs
Inoculated 5mL of 1x LB + Kan50 (made by Steven on 3/23/11). Incubated O/N at 37C, 250RPM. Will perform mini preps tomorrow. The following samples were selected:
- MM09 – #1, 2, 8
- MM11 660bp – #1, 2, 8
- MM10 2/8/11 – #1, 2
- MM04 1/19/11 – #2, 3
- MM11 3000bp – #3
- MM04 1500bp – #4
- MM06 1/19/11 – #1, 2
- MM04 550bp – #1, 2
- MM05 1/19/11 – #1, 2
Mini Preps – Liquid Cultures from yesterday
Mini prepped 3mLs of each culture, according to Qiagen protocol. Samples were eluted with 50uL of Buffer EB.
- #9
- #10
- #13
- #43
- #45
- #49
- #56
- #58
Bacterial Cultures – Colonies Selected by Steven from Steven’s Re-Streaked Plate
Inoculated 5mL of 1x LB + Kan50 (made by Steven on 3/23/11). Incubated O/N @ 37C, 250RPM. Will perform mini preps tomorrow. The following samples were selected (red text on the plate):
- #9
- #10
- #13
- #43
- #45
- #49
- #56
- #58
Colony PCR – Colonies from COX1 Genomic Cloning (from 20110411)
Ran colony PCR on various colonies produced from cloning on 20110411. All colonies were picked, re-streaked on Kan50 plate(s) and PCR’d. Master mix calcs are here. Cycling params:
- 95C – 10mins
40cycles of:
- 95C – 30s
- 55C – 30s
- 72C – 3mins
- 72C – 10mins
Results:
Colony PCR – 5’RACE Colony: COX2 (repeat of yesterday’s PCR)
Repeated yesterday’s PCR on the re-streaked colony in order to run the product on a gel with a more appropriate ladder. See yesterday’s entry for all PCR info.
Results:
Lane 1: Hyperladder I
Lane 2: colony PCR
Lane 3: NTC
A band of nearly ~950bp is seen in the colony PCR, suggesting that the cloning reaction was successful. However, this does not match up with the expected size of ~1500bp seen on 20110407. Will sequence this regardless. Also, the gel on 20110407 may not have run properly (see image from that dat), which could possibly explain why we don’t see the “expected” size band of ~1500bp? Will inoculate a liquid culture for mini prep for eventual sequencing.
Colony PCR – 5′ RACE Colony: COX2
One white colony (marked with arrow in image linked) from the two plates from Steven’s cloning (from yesterday) was picked, restreaked on a new Kan50 plate (no X-gal) and PCR’d.
Master Mix:
2x Apex Red Master Mix – 25uL
10uM M13 Forward – 1uL
10uM M13 Reverse – 1uL
H2O – 23
Added 25uL to each PCR tube.
Cycling Params:
- 95C – 10mins
40 cycles of:
- 95C – 30s
- 55C – 30s
- 72C – 2mins
1 cycle:
- 72C – 10mins
Results:
Lane 1: Hyperladder IV
Lane 2: colony PCR
Lane 3: NTC
Turns out the Hyperladder IV (this gel was run in the Friedman Lab) only goes up to 1000bp. So, the band we see in the colony PCR reaction could be close to the expected size if the insert is present (~1500bp). Although, we also see a band in the NTC. Will repeat this PCR and run on a gel with a more appropriate ladder…