Team:EpiphanyNYC/Notebook

Notebook

 

Week 1 (March 19-25)

  • Consulted with our advisor, Frank, to advise researchers and scientists
  • Reached out to scientists at Mt Sinai Hospital, Jason Fuller and Russell Hanson
  • Met with Jason Fuller and Russell Hanson, scientists at Genetics Department at Mt Sinai Hospital
  • Scheduled weekly meetings for the rest of the year

Week 2 (March 26-Apr 1)

  • Brainstormed for a potential topic (Sickle Cell Anemia, Cystic Fibrosis, Huntington’s Disease); decided on HD, proposed by Yeji Cho
  • Determined project leaders of the project
  • Divided into subsections (website, design, fundraising, social media, computational) and assigned roles, such as other team leads

Week 3 (Apr 2-8)

  • Determined possible method to target the disease
  • Outlined the abstract for the project

Week 4 (Apr 9-15)

  • Took headshots of members and team pictures to put on website
  • Administered Drug Tests for medical clearance
  • HIPAA (Health Insurance Portability and Accountability Act) Training
  • Fire Drill Practice

Week 5 (Apr 16-22)

  • Decided to use WordPress as website template
  • Happily received our lab coats and Mount Sinai IDs

Week 6 (Apr 23-29)

  • Submitted payment for iGEM group registration
  • Signed consent forms

Week 7 (Apr 30-May 6)

  • Designed graphic of brain and neuron for website

Week 8 (May 7-13)

  • Brainstormed for a team name and designed logo; decided on HD Resolution

Week 9 (May 14-20)

  • Designed T-shirts, hats, and sweaters
  • Brainstormed for companies/sponsors to partner with us
  • Received iGEM parts kit

Week 10 (May 21-27)

  • Organized home page of website
  • Created sponsorship/partnership letters for possible companies

Week 11 (May 28-Jun 3)

  • Julia, Erik and Stacy organized a table at Peace Angels Benefit Concert at Steinway and Sons Concert Hall in May 28, 2017
  • Mailed out consent forms
  • Scheduled wetlab training dates for the summer

Week 12 (Jun 4-10)

  • Early Training: lab safety, project overview, practiced lab techniques such as pipetting, centrifugation, PCR, etc.

Week 13 (Jun 11-17)

  • Organized team page of website
  • Contacted over 50 private and public companies in pharmaceutical and biotech industries, non-profit organizations for sponsorship and support.

Week 14 (Jun 18-24)

  • Created Twitter account
  • Christi and Marianne completed safety form 1, 2, 3

Week 15 (Jun 25-Jul 1)

  • Jason, Justin, Jeewhan, Marianne met up to analyze the data collection

Week 16 (Jul 2-8)

  • Computational Lab Weeks:
  • First weeks we talked about how to get an application called mFold
  • mFold helps to create a simulation of the RNA bonds fusing instead having to actual do it experimentally

Week 17 (Jul 9-15)

  • Computational Lab Weeks (continued):
  • Looked for Huntington’s mRNA in particular in NCBI
  • NM numbers, other prefixes gave types of mRNA
  • HW: Find huntington’s-related sequences in NCBI database (assumed at least 5-10 sequences)

Week 18 (Jul 16-22)

  • Christi, Rachel, Esther, and Marianne organized a fundraising and information table at Dominico-American Society of Queens in Flushing Town Hall in Flushing, Queens NY in July 22 2017
  • Created Facebook account
  • Created GoFundMe page

Week 19 (Jul 23-29)

  • Received over 100 likes on Facebook page thanks to our Social Media and Outreach team.
  • Computational Data:
  • We used data we received from [ncbi.com] and used it to compare with the wild type and the infected types.
  • HW Results: Found 2 accession numbers- NM_002111.8 (mRNA) and NP_002102.4 (protein); however, only one was mRNA and none were disease form
  • We then collected the data in our shared folder
  • Looked through other databases for other mutants; found:
  • Study with “20 Huntington’s Disease and 49 neurologically normal control samples from post-mortem human subjects”
  • http://trace.ddbj.nig.ac.jp/DRASearch/study?acc=SRP051844
  • Results for HTT on DNA Data Bank of Japan (includes above):
  • http://trace.ddbj.nig.ac.jp/DRASearch/query?keyword=htt&show=20&fq_rep_name=Homo%20sapiens
  • HW: Run wild-type mRNA on mfold (Create a text document with the NM_00211.8 RNA and run mFold on it http://unafold.rna.albany.edu/?q=mfold)
  • We then collected the data in our shared folder

Week 20 (Jul 30-Aug 5)

  • Ordered materials (E. coli, etc)
  • Computational Data:
  • HW Results: Nobody able to run mfold successfully locally or on web
  • Changed programs to ViennaRNA:

    HW: Re-calculate sequences with artificially added CAG repeats (added 42 and 60 repeats)

Week 21 (Aug 6-12)

  • Wrote letters to respective schools to ask for partnerships
  • Manually analyzed results of ViennaRNA calculations for chaperone/guideRNA hairpin targets.
  • Determined that this process was less reproducible than desired, and it worried the most viable hairpin loop might be buried in the the tertiary structure
  • Decided to change approach: Use RNAi tools to calculate the toe-hold footing (areas in RNA that can be used to initiate strand displacement and/or break apart mRNA secondary structures).
  • Spent remainder of the day testing the following tools:
  • We used to addgene.com to find plasmids that had less than 26Q repeats.
  • We used a genome to protein sequence converter called [] in order to compare the wild type plasmid and the infected.
  • At first we thought we had a good candidate with 20Q that was very similar, however, didn’t work because the sequence didn’t completely match up with the wild type.
  • Therefore kept looking and decided to use pEGFP-Q23 https://www.addgene.org/40261/

Week 22 (Aug 13-19)

  • Created Instagram account
  • Grew cell subcultures of E. Coli for future testing
  • Familiarized ourselves with autoclaving and basic sterilizing processes
  • Learned how to store E. coli for future experiments
  • HDSA agreed to be sponsor

Week 23 (Aug 20-26)

  • Learned about transfection and tested cells for competency
  • Updated team Wiki’s page on the iGem website
  • Reached out to our respective high schools for sponsorship
  • Hereditary Disease Foundation/Huntington’s Disease Foundation agreed to be sponsor

Week 24 (Aug 27-Sept 2)

  • Jessica, Erin, Catherine, and Yunsu helped organize a presentation table at Dominico-American Society of Queens Benefit Concert at National Opera America Center in New York NY on August 30 2017
  • Reached out to Cerebral Palsy Alliance Research Foundation about partnering and sponsorship and discussed creating a joint campaign CPARF’s Steptember campaign to promote 10,000 steps a day goal
  • Registered team members and created a team roster

 

protocol Created with Sketch.

Testing Competency of Cells

Project: HD Resolution iGEM Notebook
Authors: HD Resolution iGEM
Date: 2017-09-19
Tuesday, 9/19/17
1.
Clean working area with 10% ethanol
2.
Throw competent cells on ice
3.
Label one 1.5 mL microcentrifuge tubes for each transformation and pre-chill on ice.
a.
Orange = 50 pg/μl
b.
Yellow = 10 pg/μl
c.
Red = 100 pg/μl
4.
Spin down DNA tubes from competent cell test kit. Quick spin of 20-30 seconds at 8000-10000rpm
5.
Pipet 10μl of DNA into centrifuge tubes. 50μl of competent cells already aliquoted. Flick gentlly
6.
Incubate on ice for 30 min.
7.
Heatshock cells into water bath of 42 degrees Celsius for 45 sec.
8.
Immediately transfer tubes back into ice and incubate on ice for 5 min
9.
Add 950 μl of SOC Media per tube and incubate at 37 degrees Celsius for 1 hour, shaking at 200-300rpm.
10.
Pipet 100μl from each tube onto appropriate plate, spread mixture evenly.
11.
Incubate at 37 degrees Celsius overnight/16 hrs. Place plates with agar side on top and lid on bottom.
 

HD RESOLUTION

hdresolutionigem@gmail.com | Phone: (347) 709-6167