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Team:Freiburg Bioware/NoteBook/Labjournal
From 2010.igem.org
Get to know our virus
Our project starts with first sequence analysis.Checking iGEM compatibility
Scanning for iGEM restriction sites:• Vector plasmid
• Thymidine kinase
• Cytosindeaminase
First practical steps
We took a closer look to the theoretical DNA- and amino acid sequence of the ITRs, questioned the role of the β-globin intron, had a closer look to the CMV promoter and performed our first cloning attempt.First fluorescing HT1080 cells
We conducted our first site-directed mutagenesis.First cell culture steps:
• Splitting and seeding of AAV 293 and HT1080 cells
• Calcium phosphate transfection
• Transduction with virus particles containing YFP encoding sequence
• Microscopy: Fluorescent transduced HT1080 cells
We planned to determine infectious virus titer via quantitative real-time PCR. For this purpose primers were designed, transduced HT1080 cells were harvested and prepared.
Theoretical studies of the AAV structure: Impressions.
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https://2010.igem.org/Team:Freiburg_Bioware/NoteBook => Back to Notebook overview]
- March (labday 1)
- April (labday 2 - 5)
- May (labday 6 - 17)
- June (labday 18 - 45)
- July (labday 46 - 75)
- August part 1 (labday 76 - 92)
- August part 2 (labday 93 - 106)
- September part 1 (labday 107 - 123)
- September part 2 (labday 124 - 135)
- October part 1 (labday 136 - 149 )
- October part 2 (labday 150 - 166 )
- November (labday 167 - 170 )
- Cellculture
