Team:USTC CHINA/Notebook/Protocols/Sample analysis

From 2013.igem.org

(Difference between revisions)
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<h1>Sample analysis</h1>
<h1>Sample analysis</h1>
<p>Sample analysis
<p>Sample analysis
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1. Preparation of soluble and insoluble cell extracts from B. subtilis
+
1. Preparation of soluble and insoluble cell extracts from B. subtilis</br>
-
- harvest cells by centrifugation (10 min, 6,000 x g, 4 °C)
+
- harvest cells by centrifugation (10 min, 6,000 x g, 4 °C)</br>
-
- wash and resuspend in 50 mM sodium phosphate buffer (pH 7.0) at an OD600 of 10
+
- wash and resuspend in 50 mM sodium phosphate buffer (pH 7.0) at an OD600 of 10</br>
-
- disrupt cells by ultrasonication (12 W, 6 x 15 pulses with 15 sec intervals) in 1.5 ml
+
- disrupt cells by ultrasonication (12 W, 6 x 15 pulses with 15 sec intervals) in 1.5 ml</br>
-
Eppendorf tubes containing 1 ml of cell suspension, supplemented with lysozyme
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Eppendorf tubes containing 1 ml of cell suspension, supplemented with lysozyme</br>
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(250 μg/μl, CB-0663-5GAM), on ice
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(250 μg/μl, CB-0663-5GAM), on ice</br>
-
破碎1:超声  
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破碎1:超声</br>
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- alternatively, cells can be disrupted by beat beating:
+
- alternatively, cells can be disrupted by beat beating:</br>
-
disrupt three times with glass beads (0.1 mm in diameter) (1 g/ml of cell suspension) in
+
disrupt three times with glass beads (0.1 mm in diameter) (1 g/ml of cell suspension) in</br>
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an orbital mixer at 180 V, with the mix kept on ice for 3 min between each disruption
+
an orbital mixer at 180 V, with the mix kept on ice for 3 min between each disruption</br>
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破碎2:玻璃珠机械破碎
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破碎2:玻璃珠机械破碎</br>
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- take 100 μl of the preparation as first total protein sample (T1)
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- take 100 μl of the preparation as first total protein sample (T1)</br>
-
得到T1
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得到T1</br>
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- remove cell debris by centrifugation at 4,300 x g, 10 min
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- remove cell debris by centrifugation at 4,300 x g, 10 min</br>
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- take 100 μl of the supernatant for the second total protein sample (T2)
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- take 100 μl of the supernatant for the second total protein sample (T2)</br>
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- spin at 8.200 x g (10 min, 4 °C)  
+
- spin at 8.200 x g (10 min, 4 °C) </br>
-
to separate into insoluble (I) and soluble (S) protein fractions.
+
to separate into insoluble (I) and soluble (S) protein fractions.</br>
-
- per sample use the amount of protein corresponding to 0.025 of OD600 for separation by
+
- per sample use the amount of protein corresponding to 0.025 of OD600 for separation by SDS-PAGE</br>
-
SDS-PAGE
+
- analyze samples by immunoblotting with specific antiserum</br>
-
- analyze samples by immunoblotting with specific antiserum
+

Revision as of 14:43, 25 September 2013

Sample analysis

Sample analysis 1. Preparation of soluble and insoluble cell extracts from B. subtilis
- harvest cells by centrifugation (10 min, 6,000 x g, 4 °C)
- wash and resuspend in 50 mM sodium phosphate buffer (pH 7.0) at an OD600 of 10
- disrupt cells by ultrasonication (12 W, 6 x 15 pulses with 15 sec intervals) in 1.5 ml
Eppendorf tubes containing 1 ml of cell suspension, supplemented with lysozyme
(250 μg/μl, CB-0663-5GAM), on ice
破碎1:超声
- alternatively, cells can be disrupted by beat beating:
disrupt three times with glass beads (0.1 mm in diameter) (1 g/ml of cell suspension) in
an orbital mixer at 180 V, with the mix kept on ice for 3 min between each disruption
破碎2:玻璃珠机械破碎
- take 100 μl of the preparation as first total protein sample (T1)
得到T1
- remove cell debris by centrifugation at 4,300 x g, 10 min
- take 100 μl of the supernatant for the second total protein sample (T2)
- spin at 8.200 x g (10 min, 4 °C)
to separate into insoluble (I) and soluble (S) protein fractions.
- per sample use the amount of protein corresponding to 0.025 of OD600 for separation by SDS-PAGE
- analyze samples by immunoblotting with specific antiserum