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PROTEIN RECEPTOR GROUP


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Overview: 

The plaques found in the brain of a patient with Alzheimer's disease comprise beta-amyloid protein oligomers, which are responsible for the degenerative symptoms of the condition. In order to diagnose and/or treat Alzheimer's disease, we must first be able to detect the presence of these beta-amyloid oligomers. One of the possible methods of detection is the use of beta-amyloid oligomer-specific transmembrane receptors.

Leukocyte immunoglobulin-like receptor (LilrB2) and its murine homolog Paired Immunoglobulin-like Receptor B (PirB) are trans-membrane receptors capable of selectively binding beta-amyloid oligomers (of x or more monomers). It belongs to a family of proteins that bind to MHC1 molecules on antigen presenting cells and is only expressed in monocytes and B-cells (and at lower levels in dendritic cells and natural killer cells) in humans. When beta-amyloid oligomers bind to the extracellular domain of LilrB2, it is activated and then goes on to recruit cofilin to its intracellular domain. 

In our proposed detection model, we would construct a fusion protein where a linker, TEV protease cleavage site and transcription factor (in that order) are fused to the intracellular domain of LilrB2. We would also fuse a TEV protease to cofilin. In that way, when beta-amyloid oligomers bind to the receptor, thus activating it, the TEV protease on the recruited cofilin cleaves at the cleavage site releasing the transcription factor in to the cytosol. The cleaved portion will be guided to the nucleus of the cell and will go on to activate the subsequent processing module.

 

 
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To Do:

  •  Run gel on PCR products - gel extraction
19/7
  •  Send PirB pEXPRs for sequencing
19/7
  •  Miniprep cofilin liquid cultures
19/7
  •  Run gel on digested PirB pEXPRs
19/7
  •  Miniprep correct pEXPR_hEF1a:PirB
19/7

 

Construction Plan

Experiments:

 

A Testing membrane localization of receptor protein

B Testing oligomer binding to receptors

C Comparing levels of endogenous and exogenous cofilin

D Testing TEVp-Cofilin cleavage with inactive receptors

E Testing TEVp-Cofilin cleavage with active receptors

F Whole system characterization

G Evaluating production of abeta by HEK293-APPSwe

 

 

 

 

 

 

 

 

Experimental Outline:

GroupDescriptionExperiments Included
ATesting membrane localization of receptor proteinA1, A2,
BTesting oligomer binding to receptorsB1, B2
CComparing levels of endogenous and exogenous cofilin 
DTesting recruitment of cofilin to the activated receptors 
EWhole system characterization 

 

 

 

 

 

 

 

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August 23 + 24

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August 31

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titleSeptember

September 1 + 2

September 3 + 4

Sep 8

 

 

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TO DO (cloning things):

  •  LilrB2 PCRs (didn't work (sad))
8/18
  •  LR hEF1a and TRE LilrB2
    •  Pick LilrB2 golden gate colonies --> LilrB2 pENTR
    •  Miniprep LilrB2 pENTR
    •  Run digest on LilrB2 pENTR
    •  Send LilrB2 pENTR for sequencing
    •  If digest looks good: LR hEF1a: and TRE: LilrB2
    •  Transform
    •  Pick pEXPR hEF1a:LilrB2 and TRE:LilrB2
    •  Miniprep pEXPR hEF1a:LilrB2 and TRE:LilrB2
    •  Run digest on ^
    •  If digest looks good, innoculate for midi
    •  Midiprep hEF1a:LilrB2 and TRE:LilrB2
  •  8/21
  •  8/22
  •  8/22
  •  8/22
  •  8/22
  •  8/23
  •  8/24
  •  8/25
  •  8/26
  •  8/26
  •  8/26
  •  8/29
  •  Verify pEXPR hEF1a:PirB-YFP is actually a pEXPR - do the LR if it's not
8/21
  •  LR PirB-YFP with TRE
 
  •  Pick LilB2YFP/TCS colonies
  •  Miniprep + digest

For LilrB2TCS only:

  •  Send for sequencing
  •  LR (hEF1a + TREt)
  •  Transform
  •  Pick colonies
  •  Miniprep
  •  Digest
  •  TREt with XbaI (CS)
  •  hEF1a with ApaI (CS)
  •  Midiprep

8/28
8/29

 

8/29
9/3
9/4
9/5
9/6
9/6
9/7

 

 

 

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