Difference between revisions of "Part:BBa K608013"

Revision as of 11:08, 21 September 2011

strong Promoter with strong RBS and RFP

This part consists of a strong promotor with strong RBS and tagged with RFP to quantify the expression.

The RFP fluorescence was measured with a plate reader:

The fluorescence intensity and protein concentration were measured with the FLUOstar Omega,
which is a multi-mode microplate reader. Samples were pipetted into the microplate and analyzed via the plate reader. In this experiment we focused on the protein concentration and the fluorescence intensity of RFP. We measured the protein concentration with the bradford-assay. This is a method to determine the total protein To analyze the protein concentration of the samples, Coomassie Brillant Blue was pippeted to each sample. With the binding of the dye to the proteins the color changes from dark red to blue. The more protein in the solution the more Coomassie dye can bind to proteins and the more the color changes into blue. The absorption of bound Coomassie dye is 595nm. The absorbance is proportional with the amount of bound dye. With a series of Bovine Serum Albumin (BSA) measurements the exact protein concentration of the samples can be determined. BSA acts like a “marker” because the concentration of BSA is known and with a linear calibration line the exact protein concentration can be detected.

With RFP (Red Fluorescence Protein) the activity of promotor and RBS can be quantified. RFP served like GFP as a reporter to determine the expression level. RFP is excited at a wavelength of 580nm. The more RFP in the solution the more is the RFP fluorescence intensity.The plate reader illuminates the samples with a high energy xenon flash lamp. Optical filters or monochromator create the exact wavelength. The more GFP in the sample the higher is the GFP fluorescence intensity. The intensity is collected with the second optical system and is detected with a side window photomultiplier tube.

RFP fluorescence intensity dependent on the strenght of promotor and RBS

sample	PR1	PR2	PR4	PR5	PR6
RFP fluorescencen intensity	25310.5	27144.5	9675,1	13415,9	685,6
factor	36,9	39,6	14,1	19,6	1,0

Sequence and Features

Assembly Compatibility:

10
COMPATIBLE WITH RFC[10]
12
INCOMPATIBLE WITH RFC[12]
Illegal NheI site found at 7
Illegal NheI site found at 30
21
COMPATIBLE WITH RFC[21]
23
COMPATIBLE WITH RFC[23]
25
INCOMPATIBLE WITH RFC[25]
Illegal AgeI site found at 616
Illegal AgeI site found at 728
1000
COMPATIBLE WITH RFC[1000]

@@ Line 5: / Line 5: @@
 The RFP fluorescence was measured with a plate reader:<br/>
-[[Image:Freiburg2011_BSA.jpg|right|350px|BSA calibration line]]
+[[Image:Freiburg2011_BSA.jpg|right|350px|caption|BSA calibration line]]
 The fluorescence intensity and protein concentration were measured with the FLUOstar Omega, <br/>
 which is a multi-mode microplate reader.
@@ Line 15: / Line 15: @@
 With RFP (Red Fluorescence Protein) the activity of promotor and RBS can be quantified.
 RFP served like GFP as a reporter to determine the expression level. RFP is excited at a wavelength of 580nm. The more RFP in the solution the more is the RFP fluorescence intensity.The plate reader illuminates the samples with a high energy xenon flash lamp. Optical filters or monochromator create the exact wavelength. The more GFP in the sample the higher is the GFP fluorescence intensity. The intensity is collected with the second optical system and is detected with a side window photomultiplier tube.
-[[Image:Freiburg2011_RFP-PR1.jpg|left|400px|RFP fluorescence intensity dependent on the strenght of promotor and RBS]]
+[[Image:Freiburg2011_RFP-PR1.jpg|left|400px|caption|RFP fluorescence intensity dependent on the strenght of promotor and RBS]]
+{|cellpadding="10" cellspacing="0" border="1"
+|sample
+|'''PR1'''
+|PR2
+|PR4
+|PR5
+|PR6
+|-
+|RFP fluorescencen intensity
+|'''25310.5'''
+|27144.5
+|9675,1
+|13415,9
+|685,6
+|-
+|factor
+|36,9
+|39,6
+|14,1
+|19,6
+|1,0
+|}
 <br/>
 <br/>