IGEM:MIT/2005/Sensor 2

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Revision as of 01:44, 22 July 2005 by >Aanniev (→‎Open Issues/Questions)
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POC

FecAnnie

Office: BUG Lounge
Email: aanniev@mit.edu
Phone: 617-252-1680
X5-6256 (dorm)

Function

  • Main component: FecA protein
  • Purpose: fusion with scFv
  • Mechanism: ligand binds to scFv induces conformational changes in FecA protein --> PoPS

Device Depiction

File:Receiver.2.FecA.ppt

Device Parts

  • Specified:
  1. FecA gene BBa_J07017
  2. FecA' (w/out PstI) BBa_J07018
  3. FecA promoter BBa_J07019
  4. FecI gene BBa_J07022
  5. FecR gene BBa_J07021
  6. FecR' (w/out PstI) BBa_J07023
  7. GFP under FecA promoter BBa_J07034
  8. Test construct for FecA BBa_J07035
  • Biobricking: all base components

Current Status

Done with

  • Primers:
  1. native FecA
  2. to point-mutate FecA
  3. FecA promoter
  4. FecI
  5. FecR
  6. to point-mutate FecR
  • Experiment read out
  • Cells:
  1. FecA+ (MC4100)

Working on

  • Redesign FecA promoter primers
  • Design primers for internal fusion
  • Spec out FecA-scFv
  • LambdaRed to make our own FecA-
  • Obtain Fur- from Boston Medical Center -- POC Ray
  • Specifying composite parts

Open Issues/Questions

  1. Linker design
  2. FecA, FecI, and FecR same promoter have issues?
  3. Delete loops that's not necessary to make the FecA-scFv work
  • [[../Issues solved/]]

Need Help With

  • Need to do:
  1. Internal fusion
  2. Get Fur- -- Work w/ Ray
  3. Make FecA-
  • Need opinions/knowledge/expertise:
  1. FecA, FecI, and FecR relationship w/ respect to control of one promoter
  2. Alternative methods for gene fusion: random mutation by circular permutation and XL1-Red

Experiments

META LEVEL

1.Build

(a) [[../Fuse FecA with scFv/]] at chosen points and attach chimera to known promoter (makes promoter::FecA::scFv)
(b) Attach FecA promoter with reporter(GFP) - makes FecApromoter::GFP
(c) If needed put FecI and FecR under a known promoter.


2.Tests Test expression of (b):

  • Transform FecA- strain:
FecApromoter::GFP --> Nothing
FecApromoter only --> Nothing
GFP only --> Nothing
  • Transform wt strain:
FecApromoter::GFP --> light up
FecApromoter only --> nothing
GFP only --> nothing

3. Transform FecA- strain with 1(a), (b) and (c), or 7
4. Test scFv expression in outer membrane: Detect TAG by Ab*fluorophore --> centrifuge --> FACS

FecA::scFv::TAGFecA (no scFv)FecA::scFvFecA::TAG/OmpA::TAG
FluorescenceYesNo (-ve control)No (-ve control)No (+ve control)

5.Test overall system: (Negative controls: no GFP under promoter, no scFv, wt FecA strain)

+ Fluorescein- Fluorescein To Do Next
GFP produced No GFP produced System works!! --> Characterize system
Anything else Anything else Go To 6.

6. System doesn't work. Troubleshoot. Test binding of antibody with antigen (FRET etc). If ok, then:
(a) Either choose a new point to fuse scFv with FecA. Go to 1.
(b) Introduce random mutations. Go to 7.

7. Miniprep plasmid DNA and insert random mutations (by either transposons/Drew's paper/circularization). Go to 3.

TIME SCHEDULE

July Week 3
   *Make stock of WT FecA, FecA promoter, FecI, and FecR
    Make FecA' 
   *Assemble FecA promoter with GFP
   *Order: primers for gene sequences for fusion 
   *Obtain: Fur-

July Week 4 
   *Make FecR' 
    Make FecA-
   *Make FecA-scFv fusions

Aug Week 1
   *Finish making FecA-scFv fusions
   *Assemble parts

Aug Week 2
   *Finish assembling parts

Aug Week 3

Aug Week 4

[[../Annie's Notes/]]

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