Edinburgh/11 August 2008

From 2008.igem.org

(Difference between revisions)
(New page: <html> <head> <title>Edinburgh iGEM 2008</title> <script type="text/javascript"> //Drop Down Tabs Menu- Author: Dynamic Drive (http://www.dynamicdrive.com) //Created: May 16th, 07' var ta...)
(Monday 11 August 08)
Line 301: Line 301:
* '''M109-M112''' Minipreps of pSB1A2+''crtB''+''crtI'', from plates 102. '''M113-M116''' Minipreps of pSB1A2+''glgC''-mut1,2 from plate 103. '''M117-M120''' Minipreps of pSB1A2+''glgC''-mut1,2,3 from plate 94 (OG)
* '''M109-M112''' Minipreps of pSB1A2+''crtB''+''crtI'', from plates 102. '''M113-M116''' Minipreps of pSB1A2+''glgC''-mut1,2 from plate 103. '''M117-M120''' Minipreps of pSB1A2+''glgC''-mut1,2,3 from plate 94 (OG)
* Double digestion of M109 to M120 with EcoRI/PstI, run on '''gel 44'''. M110-102 (pSB1A2+''crtB''+''crtI'') have a band at 2.5kb as expected. M109 (pSB1A2+''crtB''+''crtI'') gave a band at 3kb instead, so should be ignored from now on. (Yan)
* Double digestion of M109 to M120 with EcoRI/PstI, run on '''gel 44'''. M110-102 (pSB1A2+''crtB''+''crtI'') have a band at 2.5kb as expected. M109 (pSB1A2+''crtB''+''crtI'') gave a band at 3kb instead, so should be ignored from now on. (Yan)
 +
* Subbed white colonies from plates 105 (pSB1A2+''crtY'') and 106 (pSB1A2+rbs+''crtY'') to '''Plate 108'''. (CF)

Revision as of 12:13, 28 August 2008

Edinburgh iGEM 2008

 

Week 9

Monday 11 August 08

  • PCR products of P55 to P58 (cenA and cex) were run on Gel 41: cex with KOD polymerase (P57) generated a single band of the desired size. However, cex with Velocity polymerase and cenA with both KOD or Velocity polymerase failed. (YAN)
  • PCR products P61 to P63 (rrnB, cenA, cex) were run on Gel 42. Very clear band for rrnB, no bands for either cenA or cex. (CF)
  • Made Plate 109/110 (Transformation of L33: pBS1A2+pCstA), 111/112 (transformation of L34: pBS1A2+dxs+crtE) and Plate 113/114 (Transformation of L35: pBS1A2+dxs+lims1). (Yan)
  • Maxipreps X9 of pSB1A2+rbs+dxs (as for M72) and X10 of pSB1A2P+rbs+appY (as for M82). (AM)
  • Redid PCR (KOD) of cex from C. fimi genomic DNA but with 10µl 50% glycerol, denaturing 1 min, annealing 60°C for 30s and extension 30s (P64). To be run on gel tomorrow. (AM)
  • Digested P57 (cex from KOD PCR) with EcoRI/PstI to confirm identity of the gene. cex has a PstI restriction site near its midpoint, so this digestion should generate two segments of approximately 750bp. To be run on gel tomorrow. (AM)
  • Digests performed using EcoRI/PstI to move crtE from BABEL2 (M79) to Edinbrick1. In each case, 3µl of vector was digested in 20µl total volume. The digests were run on a gel ready for excision, but gel showed no band corresponding to crtE (see gel 43 showing a single band at ~3kb for BABEL2+crtE and bands at ~2.5kb and 800bp for Edinbrick1). (AH)
  • M109-M112 Minipreps of pSB1A2+crtB+crtI, from plates 102. M113-M116 Minipreps of pSB1A2+glgC-mut1,2 from plate 103. M117-M120 Minipreps of pSB1A2+glgC-mut1,2,3 from plate 94 (OG)
  • Double digestion of M109 to M120 with EcoRI/PstI, run on gel 44. M110-102 (pSB1A2+crtB+crtI) have a band at 2.5kb as expected. M109 (pSB1A2+crtB+crtI) gave a band at 3kb instead, so should be ignored from now on. (Yan)
  • Subbed white colonies from plates 105 (pSB1A2+crtY) and 106 (pSB1A2+rbs+crtY) to Plate 108. (CF)