Difference between revisions of "Team:ICT-Mumbai/Notebook"

Week 2: Ground Reality

During this week, we decided to approach different NGOs and organizations that are involved in promoting and providing better sanitation. Sulabh International is an India-based NGO that promotes and provides better sanitation by building public pay and use toilets and community toilets. To understand and evaluate the feasibility of our idea and to understand the ground reality, we decided to meet with a representative of Sulabh International. Details of our interaction with this NGO can be found on our human practices page.

Week 4:The idea!

Glutamine synthetase (glnA), and the smaller and bigger subunits of glutamate synthetase (gltD and gltB, respectively) were our genes of primary interest. All the three genes of interest were amplified from E. coli BW25113 genomic DNA using polymerase chain reaction (PCR). PCR products were loaded and run on 1% agarose gel to check for the correct sizes of these three genes (glnA: 1640 bp, gltB: 4462 bp, gltD: 1420 bp). Among the three, we were successful in obtaining two genes — glnA and gltD. We repeated PCR for gltB for the second time by adding DMSO. This time too we could not see bands of correct size. We again carried out PCR using different annealing temperatures and the product obtained with 62°C as annealing temperature gave good bands. This was further gel purified and used as a template to carry out another PCR for the same gene. We could not see bands of correct size again.

Week 6: We don't give up!

We repeated PCR for gltB using a different polymerase enzyme — Long PCR Enzyme Mix (Thermo Scientific #K0182).
We checked for the correct band (4462 bp) using agarose gel electrophoresis . Hurray! Positive results finally. gltB was further gel purified and RE digested with SalI and SmaI. pUC19 was digested with BamHI. Digested pUC19 was gel purified and digested gltB was PCR purified and a ligation reaction of both was was set up in 1:3 molar ratio. We sent out all three genes for sequencing.

Week 8: Making way for proteorhodopsin!

In order to make the GS-GOGAT cycle work, we needed proteorhodopsin (PR) that would produce ATP with the help of the proton gradient. However, this activity of PR is seen only in the presence of retinal. We found both, the gene for PR (BBa_K773002) and a device for retinal biosynthesis (BBa_K1604022) in the provided kitplate. For PR, we decided to use an araC regulated promoter (BBa_R0080) which was also present in the kitplate.

We reconstituted BBa_K773002 (Plate 2, well 1P), BBa_K1604022 (Plate 7, well 17K), BBa_R0080 (Plate 3, well 5G) and transformed in E. coli DH5α competent cells.

Colonies were found only for BBa_K773002. BBa_K1604022 and BBa_R0080 gave no colonies. We repeated the transformation for these two parts, this time we increased the incubation time for each. We were successful.

Week 10: Gene deletions!

We learned that ammonia assimilation in E. coli is regulated by PII proteins that adenylate glutamine synthetase (GS) under nitrogen rich conditions and render it inactive. It was found that the cell also contains another PII like protein called GlnK.(Ref. 2)
Since we wanted the cells to work under ammonia rich conditions, we had to delete glnB gene coding for PII, and, glnK gene coding for glnK. Gene deletions were carried out as described by Datsenko and Wanner (Ref. 3).

Week 12: 3A assembly!

Sequencing results were positive only for glnA We carried out a variant of 3A assembly using BBa_1604022 (cut with EcoRI and SpeI), BBa_I74211(cut with XbaI and PstI) and BBa_JO4450 (cut with EcoRI and PstI). Unfortunately, it did not work.
Meanwhile, we received our gBlocks for glnA, gltDand rbs+PR from IDT. The concentrations of each of them were found to be extremely low that we reordered all the theree gblocks again.


From left to right: glnA fragment 1 (G1_F1), glnA fragment 2 (G2_F2), gltD fragment 1 (G3_F1), gltD fragment 2 (G3_F2), rbs+PR follwed by 1kb DNA ladder in the last lane.

Week 14: Examination time!

We could not work this week as our university mid-semester examinations were scheduled.

Week 16: Starting anew!

We cloned glnA in pET 43.1b vector between sites NdeI and HindII. While waiting for indC parts, we discussed about possible collaborations with other teams and started working on the team wiki>

Week 18: Getting glnA in place!

Since the concentration of G1_F1 obtained from IDT was very low, we PCR amplified it using Phusion polymerase.


From left to right: G1_F1, G1_F2 followed by 1kb DNA ladder

In the end, we determined the concentrations of G1_F1 and G2_F2 and carried out gene SOEing to join both the fragments. We did not get bands of the correct size (1640bp). We repeated gene SOEing with Pfu polymerase but to no avail.


Image of SOE PCR carried out usig Pfu

Meanwhile, we transformed BBa_K1152013 in E. coli DH5-α which gave us blue colonies after 48 hours as reported by the Heidelberg team.

Week 20: On our toes!

We immediately designed and ordered primers to amplify the ychH promoter from E. coli MG1655 genomic DNA. The ychH promoter was inoculated in LB+Kanamycin and miniprepped the next day.We await our primers!

Meanwhile, ligated products (glnA + T7 + lacI with pSB3C5) were transformed in E. coli DH5-α. Three colonies were picked up randomly and inoculated in LB+chloramphenicol. Along with that, E. coli DH5-α transformed with BBa_K1152013 was also inoculated in LB+chloramphenicol.Both were miniprepped the next day.Both were double digested with EcoRI and PstI and a ligation reaction was setup in 1:3 molar ratio. This ligated product was transformed in E. coli DH5-α. Many red colonies were seen the next day which indicate self-ligation. Other colonies were screened and found to be negative

Week 22: Our part is ready!

Screening results for all eight colonies were positive!


From left to right: Gel1_Lanes 1-5: Colony number 1-5, lane 7: Positive control, lane 8: 1kb DNA ladder, Gel2_Lanes 1-3: Colony number 6-8, lane 7: Positive control, lane 8: 1kb DNA ladder. We determined the concentration of each of these using Nanodrop spectrophotometer.

Submission: Based on the concentration obtained, we added 11ul of miniprepped DNA prep (Colony 1: pSB1C3+ychH promoter) to A1 of the 96 well submission plate, covered it with the provided lid and kept it for overnight drying. Drying was carried out in the lab’s laminar flow hood which was surface sterilized with 90% ethanol. The miniprepped DNA had completely dried in the wellthe next day. We submitted our part as per the instructions given on the iGem submission page