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Overview

B-cell receptors (BCRs) are unique in their ability to recognize a highly specific antigen and produce an intracellular response. Centering around a membrane-bound IgM antibody which performs the actual antigen detection, they also contain a number of helper proteins, in particular the membrane proteins CD79A and CD79B; inside the cell, protein kinases such as Lyn attach to their intracellular domains to receive any signal it transmits. For this project, we plan to engineer a BCR to respond to the beta-amyloid plaques that are the hallmark of Alzheimer's disease. Normally, when an antigen binds to the IgM part of the BCR, CD79A and CD79B become phosphorylated with the help of Lyn, thus recruiting another protein kinase known as Syk. In B cells, this leads to a signaling cascade which induces cell proliferation. In our circuit, we would like the binding of beta-amyloid to transmit a signal in the form of a transcription factor to our diagnosis/treatment module - although this cuts out the signal amplification resulting from the kinase cascade, it leads to a far more controlled and quantifiable cellular response. Our solution involves TEV protease, which cleaves a particular amino acid sequence (TEV cleavage site) that can be used as a linker in fusion proteins. In our system, CD79A and CD79B are linked to transcription factors by TEV cleavage sites and Syk is fused to a TEV protease. When Syk is recruited to the BCR upon beta-amyloid binding, the attached TEV protease will come in close proximity to its cleavage site, where it can cut and release the attached transcription factor into the cell. This transcription factor can then go on to activate the genes involved in our diagnosis/treatment module. Additionally, by a simple substitution our modified BCR could be adapted to detect any antigen (and release any transcription factor), making it a particularly useful synthetic biology tool.

Alternative Uses

Can sense anything

Of potential use to DoD: sensors for bio terrorism. Take our amplification testbed circuit, throw in sensors for biological weaopons. If there is a biological attack, you would find out way before symptoms develop. Keeping cells alive is relatively cheap (especially if this works in yeast), should be cheap enough to roll out. Could also potentially make antibodies to certain chemical agents.

To Do

Monday morning

Monday afternoon

pick colonies from gibsons

retransform Lyn, all the TRE parts.

Cloning

Sequence A4/B4
- A4/B4 1 and 3
fix the other Gibsons
midi culture TRE:BCR (TRE:CD79A,TRE:CD79B,TRE:GmabL,TRE:GmabH 1,TRE Lyn-mKate)
- midi prep
re digest hef1a:Lyn
appSWE?

Pick colonies from APP, APPSwe

Gibsons shouldn't exceed 30C, they are big and will recombine strangely at 37

Monday

Tissue Culture
- Seed 3 plates (2 w/ glass cover slips 1 standard)
- Dilute remaining DNA
- Update Experiments Pages
- Experiment Timeline
Cloning Transform TRE: Lyn-mKate verified mini

TRE: Lyn-TEV LR

TRE: Gmab L verified mini

TRE: CD79B verified mini

TRE: CD79A verified mini

hEF1a: Lyn LR

TRE: Syk-eYFP LR

Pick Colonies
- A/B
- A4/B
- A/B4
- A4/B4

LR
- TRE: Gmab H

Friday

TC
- Dilute Midipreps
- Update Experiments Pages
- Experiment Timeline
- Seed
Cloning
- Plasmids Library
Thursday----------------------------------------------------------------------------------------
TC
- Dilute Midipreps
- Stain Slides
- Finish Planning
- add Dox
- Seed?
Wednesday-------------------------------------------------------------------------------------
TC
- Path Foreward
- Dilute Midipreps
- Transfect
  - Tango 2
  - Membrane Localization Dilution Microscopy