Week 2: June 5-9

Monday (06/05/17) and Tuesday (06/06/17)

The first two days of this week were spent on Wright Patt Air Force Base (WPAFB). The team members toured the two labs that they would be working in and received safety training in both. The student researchers were very excited to tour the world-class facilities on base. Multiple brainstorming discussions were also held to finalize the project idea. After the week of training, the group of students split up into 2 groups: one to work in the 711th Human Performance Wing, and one to work in the Materials Directorate. The young researchers at the 711th Human Performance Wing were tasked with sensing and response while the researchers at the Materials Directorate were tasked with packaging.

Wednesday (06/07/17)

Sense/Respond: On the first day in the lab the members made LB broth, (formula in protocol tab). Although a simple procedure, this was the first hands-on experience for the students in the lab. They then did a plasma transformation protocol using E.coli JM109 and the plasmid PRhl_GFPa1. The bacteria created was plated onto LB chloramphenicol and left in incubator (37°C), overnight. If there was growth on the plates in the morning there would a greater probability that the E. coli absorbed the plasmid. The tired but excited young researchers went home with fingers crossed.

Packaging: The lab members attended a review meeting for the Materials Lab. This is where people gave mini presentations on how their projects were going and what problems they have run into. The Packaging members and Chia considered the advantages of using different surface proteins in order to package E. coli and decided on curli. The four Packaging students searched the iGEM site for parts (cellulose binding domains, Csg A, etc) was discussed.

Thursday (06/08/17)

Sense/Respond: When they entered the lab on the second day the plates showed growth with distinctions of individual colonies. Mentor Mike Goodson ecstatically let the students know about the significance of the growth and students were relieved that their plates had grown! These colonies were used to complete the PCR protocol. The master mixture, (protocol tab) and LB broth in round bottom falcon tubes were left in the incubator (37°C), overnight. The plates were put in the refrigerator (4°C) to preserve the bacteria for future use. This protocol was used to confirm that E.coli JM109 had absorbed the plasmid PRhl_GFPa1

Packaging: The teams attended a seminar given by a professor from Northwestern. The Packaging team clarified the goals of their project by deciding to attach a cellulose binding domain to the Csg A portion of a curli protein on E. coli bacteria. In the lab, the team worked with producing agarose gel, diluting a buffer, and using these components to run gel electrophoresis on DNA samples. Additionally, the team poured LB agar plates.

Friday (06/09/17)

Sense/Respond: For the last day of the week, the students’ goal was to confirm the E. Coli had absorbed the plasmid and then perform a MiniPrep Kit to take the plasmid out of the bacteria. To accomplish this, they first learned how to create a gel and how to use the electrophoresis. The electrophoresis sends the DNA down the gel using a positive and negative charge. Under a blacklight you can see if the DNA is present. Next, the students use a QIA prep spin Miniprep Kit to take plasmid out of bacteria. The students placed one nanodrop onto spectrophotometer to measure how pure the DNA extracted is. For future experiments, the plasmid DNA would then be sent to an offsite lab to be sequenced.

Packaging: The Packaging team prepared DNA samples and analyzed the samples with the Nanodrop device. Later, the team used restriction enzymes to slice open the DNA and then ran the samples through gel electrophoresis. The project idea continued to progress with the team finding parts form the iGEM inventory and researching DNA sequences of the various parts.

Week 4: June 19-23

Monday (06/19/17)

Sense/Respond: After the weekend, the students met in the lab and initiated a second digest. They were determined to get everything measured correctly and leave minimal room for mistakes. This time around, the students were much more knowledgeable about buffers and enzymes used and proceeded carefully combining them with DNA. After the digest was complete, the young scientists began prepping another gel for electrophoresis. Everything went smoothly while the digest was completed and DNA was extracted and cut by the enzymes. Next, the students prepped the DNA by adding a loading dye and then proceeded to put it on the gel. After electrophoresis for 30 min, the gel was complete. The LabPats were able to use this downtime for updating lab journals, creating new and exciting logos, as well as continuing to work on the wiki. Next, another experienced mentor helped with analyzing the gel and cutting out the DNA from the gel. However, they were quite disappointed to learn that there were 3 bars, indicating more base pairs than expected. The mentors ensured them that the gel still worked and that they just needed to cut out the fluorescent band that was relevant. Meticulous work was done to cut out the gel, and the labpats were finally able to let out a sigh of relief once the gel was safely placed in the tube and put in the fridge to be melted down tomorrow.

Packaging:

Tuesday (06/20/17)

Sense/Respond: The students quickly resumed where they had left off to begin their gel extraction. Two different protocols were used to see which one would achieve a higher concentration. The teams were divided into Tina and Annie working with Svetlana on (QIAEX II Agarose Gel Extraction) and Jason and Dallas (who unfortunately was ill, so Annie and Tina tag teamed his sample) working with Mike on QIAEX Gel Extraction Kit. The gel extractions were performed and the nano drop test was performed. The only successful gel extractions were performed by the girls (Svetlana’s protocol), so they took home the victory! The boys learned a lot from their error and submitted defeat. The day was wrapped up by working hard designing the wiki and learning how to code.

Packaging:

Wednesday (06/21/17)

Sense/Respond: Today the students began their second Polymerase Chain Reaction (PCR). Under the watchful eye of Dr. Harbaugh, the students independently finished the PCR and loaded it into the thermocycler. Another small gel was prepared and the PCR’s were taken out and loaded on the gel. The students meticulously loaded the PCR’s onto the slits of the gel with incredible precision that truly showed their growing expertise.

The students received the results they had been hoping for, which showed that the Super folded GFP had been inserted into the bacteria. They then performed a PCR Purification, which separated the massive amounts of DNA. The DNA was then measured using the nano drop and these results were given:

Packaging:

Thursday (6/22/17)

Sense/Respond: The day began with another PCR. Today, the students were ready to completely do the PCR by themselves with little guidance from the mentors. The standard protocol was followed and the PCR and ran another cycle in the thermocycler. Meanwhile, another gel was prepared by the students. This time around, the students were very efficient and the process went by very quickly. The gel ended up giving too many bands, but the mentors conversed and decided to proceed with the PCR purification anyways. After the lab work was done, the students decided to meet with the other lab students to discuss current progress. The students created discussion points and had a great discussion with the other lab.

Packaging:

Friday (6/23/17)

Sense/Respond: The day began bright and early with two PCR digests. This time a PCR Vector Digest was conducted on the same from yesterday and a PCR GFP digest was done on the sample from Wednesday (6/21/17). After following the protocol, the students were able to successfully perform the digests. After a 2 hour wait (per the protocol), the young scientists performed a purification on the GFP digest. The goal was to cut off end bits of the base pairs to allow the plasmid connect again. During the students' lunch break, another meeting was held with teacher leaders who wanted to know information about progress and future proceedings.

Packaging:

Week 6: July 5-6

Wednesday (7/5/17)

“Ring, ring, ring!” came from the laptop as the students huddled around to receive a Skype call from the Singapore iGem team. They were greeted by Wilbert from the Singapore team. They immediately began conversing with Wilbert and exchanged project descriptions and ideas. The team was very intrigued to learn about the Human Practices components of iGem from Wilbert. After a whole hour of video conference, the team learned a lot from the sagacious Wilbert. The conversation was very beneficial to the students as they learned about the different components of iGem. Wilbert even offered to help them with the wiki page!

Sense/Respond: Afterwards, the students arrived back to the lab and received presentation tips from mentors for the upcoming lab presentations the following week.

Packaging:

Thursday (7/6/16)

Sense/Respond: The next day, the group decided to do the InterLab in order to be considered for medal criteria. They sifted through the kit and found many useful parts that they could use in order to help standardize fluorescence. After reading through the protocols and laying out a plan of attack, the students had the wait since the lab was going under routine inspection. The students spent the rest of the day designing more graphics and made wiki edits.

Packaging:

In the afternoon, the whole team got together with mentors to meet at the Air Force Museum in Dayton, Ohio in order to take self pictures and group pictures for the wiki.

Week 8: June 17-21

Monday (7/17/17)

Sense/Respond: The student sat around nervously waiting for their presentation to begin. In a few minutes they would be presenting to the whole lab about their project and goals. The students gave a phenomenal presentation that received much praise and applause. They were relieved to be done and went back to work on the wiki. Everything in the lab is up to date so the young researchers dedicated the rest of the day for wiki organization and miscellaneous tasks.

Packaging:

Tuesday (7/18/17)

Sense/Respond: Mentor Mike was finally back from vacation and the students were very excited to see him and update him on current progress. They discussed the plan moving forward and the layout of the rest of the summer. After half an hour, the students had a general idea of the "end goal". They discussed the DNA sequencing that had just come in and were like described. Afterwards the students continued working on collaboration and organizing wiki pages.

Packaging:

Thursday (7/20/17)

Sense/Respond: The day started at UES and the students began to look up literature that would help them with the sensing part of the project goal. They were able to find lots of useful information referring to the two ETEC toxins, a heat labile and heat stabile. Over the course of a couple hours, the students were able to find and compose a list of the possible ways to detect ETEC. In the afternoon, the students shared the ideas with their mentor, Mike. After lunch, the students discussed what they had gathered from the past 3 days of researching literature. After exchanging ideas and articles, the students and Dr. Goodson realized that being able to sense a quorum sensing molecule autoinducer-2 (AI-2) might be the way to go. They discussed at length the necessary components needed to be able to put the promoter into the existing plasmid so that it could detect AI-2. After a bit of research, they decided to go with E. coli DH5a which fit perfectly as it does not create AI-2 on its own. The students were relieved that they had taken a massive step forward in their “sensing” component and hope to achieve the end goal soon.

Packaging:

Friday (7/21/17)

Sense/Respond: The students finally began the lab work today for "sensing". The students worked on resuspending part K18 in Well 3 and followed the protocol to grow them up on plates. They also transformed the GFPa1 plasmid into DH5a E. coli cells. The plates were then left outside overnight to grow. Meanwhile, the young researchers were able to analyze the plasmid and look at all the restriction sites to find the ideal sites to cut the plasmid. Under the guidance of Dr. Goodson, the students picked three restriction sites and an order was put in to order the primers. Afterwards, the RH lab held their weekly lab meeting with the RX lab and shared the exciting news of their new discovery.

Packaging:

Week 10: July 31-August 4

Monday (7/31/17)

Sense/Respond: The morning started with the students performing a digest over the mini prep from several days pervious. Two digests were preformed using different sets of cut enzymes. Digest 1 was using the SpnI-HF and BmrI, while Digest 2 used the cut enzymes PacI and BmrI. The Digest was then confirmed using a gel, which showed the accurate number of base pairs.

Packaging:

Tuesday (8/1/17)

Sense/Respond: The students set up another run of their GFP Project. The students used a Kinetics reading of the Plate Reader. The kinetics were taken over 24 hours, every 20 minutes. The students then worked on the wiki, trying to create a template.

Packaging:

Wednesday (8/2/17)

Today was an exciting day for the students as they got to perform their survey at their high school. The iGEM students volunteered to help the high school on schedule pick up day. As the other students were coming to grab their schedule we would offer for them to fill out a pick survey on computers we had set up. Over 200 students varying in with some teachers filled the survey. This was a huge success for the students.

Thursday (8/3/17)

Sense/Respond: Today the students got back to work on the sense plasmid. The students performed a PCR, because finally their primers came in. The PCR product was ran on the gel and the students got the results they were hoping for. Next, they performed a MiniElute Reaction Cleanup Kit and then conducted a Nanodrop. The Nanodrop were high concentrations of DNA. To end the day, the students performed another digest using the PCR they had just purified.

Packaging:

Friday (8/4/17)

The big day to present to the Chief Scientist of the lab had finally come. Early in the day, the students had a dry presentation with their teachers and mentors. They received criticism and praise for their work and presentation that they would present later. They left in high spirits to return to the lab and begin the purification, ligation, and transformation of the plasmid for the “sense” component of the project.

Sense/Respond: The purification was then nanodroped and the students were pleased with the results. The students then performed a ligation on the plasmid backbone from the iGEM part and the sfGFP. The ligation seemed to go as planned and the students hoped that the two sticky ends had connected. After completing the transformation, they got ready to present to the Chief Scientist who got the funding for the iGem team. The presentation went extremely well and the Chief Scientist was very impressed with their work in the summer and the progress made. The students were finally able to let out a sigh of relief as they finished their presentation successfully. Afterwards, they came back to the lab to perform the transformation on the plasmid. The students followed the protocol exactly and were able to achieve favorable results.

Packaging: