Team:Grenoble-EMSE-LSU/Documentation/Notebook/August

Revision as of 00:47, 23 August 2013 (view source)

Simon.pacouret (Talk | contribs)

← Older edit

Revision as of 00:49, 23 August 2013 (view source)

Simon.pacouret (Talk | contribs)

Newer edit →

Line 26:

<h3>Thursday</h3>

<h4> KillerRed Characterization </h4>

-

<p> Tested different loading dyes enabling to follow cell viability by fluorescence microscopy. </p>

+

<p> 1) Tested different loading dyes enabling to follow cell viability by fluorescence microscopy. </p>

<h5> Materials and Methods </h5>

<p>

Line 33:

<h5> Results </h5>

<p> According to the microscopy acquisitions, Diaminofluorescein and Mitotracker Green FM do not seem to cross cell membranes. One explanation could be that the loading dye has time to leave the cell cytoplasm during the wash, between the end of the incubation and the beginning of the observation. It has to be seen if this wash process can be skipped to save time and thus increase the probability of visualizing stained cells under the microscope. </p>

-

+

</br>

-

<p> Performed a new kinetics on M15[pRep4-pQE30::KR] cells, in M9 medium. </p>

+

<p> 2) Performed a new kinetics on M15[pRep4-pQE30::KR] cells, in M9 medium. </p>

<h5> Materials and Methods </h5>

<p>

-

M15[pRep4-pQE30::KR] cells were cultured ON (37°C, 200 rpm) in 10 mL LB medium, supplemented with Kanamycin and Ampicillin. In the morning, cells were diluted 100x in fresh LB medium (with antibiotics). At OD610 = 1.5, cells were diluted 100x in 75 mL M9 medium, supplemented with 50 µg/mL Kanamycin, 200 µg/mL Ampicillin and 0.05 M IPTG. The solution was subsequently split in 3 Erlenmeyers, covered with aluminum fold, and incubated at 37°C, under light illumination. 195 min after IPTG induction, one of the Erlemeyer was uncovered, and second one followed the same fate 110 min later. OD610, fluorescence (540/630 nm) measurements and cell plating were performed every 45-70 min.

+

M15[pRep4-pQE30::KR] cells were cultured ON (37°C, 200 rpm) in 10 mL LB medium, supplemented with Kanamycin and Ampicillin. In the morning, cells were diluted 100x in fresh LB medium (with antibiotics). At OD610 = 1.5, cells were diluted 100x in 75 mL M9 medium, supplemented with 50 µg/mL Kanamycin, 200 µg/mL Ampicillin and 0.05 M IPTG. The solution was subsequently split in 3 Erlenmeyers, covered with aluminum fold, and incubated at 37°C, under light illumination. 195 min after IPTG induction, one of the Erlemeyer was uncovered, and the second one followed the same fate 110 min later. OD610, fluorescence (540/630 nm) measurements and cell plating were performed every 45-70 min.

.</p>

Team:Grenoble-EMSE-LSU/Documentation/Notebook/August

From 2013.igem.org

Revision as of 00:49, 23 August 2013

August

Week 1

Week 2

Week 3

Monday

Tuesday

Wedsnesday

Thursday

KillerRed Characterization

Materials and Methods

Results

Materials and Methods

Results

Friday

Week 4

@@ Line 26: / Line 26: @@
                                                 <h3>Thursday</h3>
                                                    <h4> KillerRed Characterization </h4>
-<p> Tested different loading dyes enabling to follow cell viability by fluorescence microscopy. </p>
+<p> 1) Tested different loading dyes enabling to follow cell viability by fluorescence microscopy. </p>
                                                       <h5> Materials and Methods </h5>
 <p>
@@ Line 33: / Line 33: @@
                                                      <h5> Results </h5>
 <p> According to the microscopy acquisitions, Diaminofluorescein and Mitotracker Green FM do not seem to cross cell membranes. One explanation could be that the loading dye has time to leave the cell cytoplasm during the wash, between the end of the incubation and the beginning of the observation. It has to be seen if this wash process can be skipped to save time and thus increase the probability of visualizing stained cells under the microscope. </p>
+</br>
-<p> Performed a new kinetics on M15[pRep4-pQE30::KR] cells, in M9 medium. </p>
+<p> 2) Performed a new kinetics on M15[pRep4-pQE30::KR] cells, in M9 medium. </p>
                                                       <h5> Materials and Methods </h5>
 <p>
-M15[pRep4-pQE30::KR] cells were cultured ON (37°C, 200 rpm) in 10 mL LB medium, supplemented with Kanamycin and Ampicillin. In the morning, cells were diluted 100x in fresh LB medium (with antibiotics). At OD610 = 1.5, cells were diluted 100x in 75 mL M9 medium, supplemented with 50 µg/mL Kanamycin, 200 µg/mL Ampicillin and 0.05 M IPTG. The solution was subsequently split in 3 Erlenmeyers, covered with aluminum fold, and incubated at 37°C, under light illumination. 195 min after IPTG induction, one of the Erlemeyer was uncovered, and second one followed the same fate 110 min later. OD610, fluorescence (540/630 nm) measurements and cell plating were performed every 45-70 min.
+M15[pRep4-pQE30::KR] cells were cultured ON (37°C, 200 rpm) in 10 mL LB medium, supplemented with Kanamycin and Ampicillin. In the morning, cells were diluted 100x in fresh LB medium (with antibiotics). At OD610 = 1.5, cells were diluted 100x in 75 mL M9 medium, supplemented with 50 µg/mL Kanamycin, 200 µg/mL Ampicillin and 0.05 M IPTG. The solution was subsequently split in 3 Erlenmeyers, covered with aluminum fold, and incubated at 37°C, under light illumination. 195 min after IPTG induction, one of the Erlemeyer was uncovered, and the second one followed the same fate 110 min later. OD610, fluorescence (540/630 nm) measurements and cell plating were performed every 45-70 min.
 .</p>