Team:WHU-China/Safety

From 2011.igem.org

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Revision as of 14:18, 26 September 2011

1st Question

1.1 Storage

1. Dried DNA: room temperature

2. Resuspended DNA: -20℃ freezer

3. The linearized plasmid backbones (25ng/ul at 50ul) should be stored at 4C or lower

1.2 Usage

1. With a pipette tip, punch a hole through the foil cover into the corresponding well to the Biobrick™-standard part that you want. Make sure you have properly oriented the plate. We recommend that you do not remove the foil cover, as it could lead to cross contamination between the wells.

2.

3. Add 10uL of diH2O (deionized water), the resuspension will become red due to the cresol red dye used during manufacturing.

4. Pipette 1 or 2uL of the resuspended DNA transform into your desired competent cells, plate bacteria with the appropriate antibiotic* and grow overnight.

5. Pick a single bacterial colony and transfer it into LB medium. Incubate the culture for 18 hours with vigorous agitation.

6. Store the single colony in physiological saline and on inclined plane, and make recognizable marks on the tube and on the notebook.

Ⅱ. Preparation of competent cells (Using Calcium Chloride)

2.1 Day 0:

Pick a single bacterial colony from a plate that has been incubated for 16-20 hours at 37℃. Transfer the colony into LB medium. Incubate the culture overnight (about 16 hours) at 37℃ with vigorous shaking.

2.2 Day 1:

1. Transfer 1 ml of the culture into 100 ml of LB medium. Incubate the culture for 2.5-3 hours at 37℃ with vigorous agitation (250-300rpm).

2. Transfer 1.5 ml of the culture into sterile ice-cold 1.5ml polypropylene tubes. Cool the cultures by storing the tubes on ice for 10 minutes.

3. Recover the cells by centrifugation at 2500 rpm for 5minutes at 4℃.

4. Decant the medium from the cell pellets. Resuspend each pellet by swirling or gentle vortexing in 100ml of ice-cold 0.1M CaCl2 solution. Store the tubes on ice for 20minutes.

5. Recover the cells by centrifugation at 2500 rpm for 5 minutes at 4℃.

6. Decant the medium from the cell pellets. Resuspend each pellet by swirling or gentle vortexing in 100ml of ice-cold 0.1M CaCl2 solution.

7. The suspension of competent cells should be immediately used in transformation.

Attention:

[1] Mix gently

[2] The newly prepared competent cells should be transformed immediately. They cannot be stored for long (except in -80℃)

[3] Keep sterile environment during operation (sterilize the clean bench by ultra-violet, sterilize hands and implements by alcohol).

[4] Use heat-shock method to transform.

2rd Question

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3rd Question

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Team:WHU-China/Safety

From 2011.igem.org

Revision as of 14:18, 26 September 2011

1st Question

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@@ Line 31: / Line 31: @@
 <h3><a href="#">1st Question</a></h3>
 	<div>
-		<p>
+		<p class=MsoListParagraph style='margin-left:36.0pt;text-indent:-36.0pt'><span
-		Mauris mauris ante, blandit et, ultrices a, suscipit eget, quam. Integer
+lang=EN-US style='font-size:15.0pt;font-family:"Times New Roman","serif"'>1.1<span
-		ut neque. Vivamus nisi metus, molestie vel, gravida in, condimentum sit
+style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
-		amet, nunc. Nam a nibh. Donec suscipit eros. Nam mi. Proin viverra leo ut
+</span></span><span lang=EN-US style='font-size:15.0pt;font-family:"Times New Roman","serif"'>Storage</span></p>
-		odio. Curabitur malesuada. Vestibulum a velit eu ante scelerisque vulputate.
-		</p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>1.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-family:"Times New Roman","serif"'>D</span><span
+lang=EN-US style='font-size:12.0pt;line-height:150%;font-family:"Times New Roman","serif"'>ried
+DNA: room temperature</span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>2.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Resuspended DNA: -20</span><span
+style='font-size:12.0pt;line-height:150%;font-family:宋体'>℃</span><span
+lang=EN-US style='font-size:12.0pt;line-height:150%;font-family:"Times New Roman","serif"'>
+freezer</span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>3.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>The linearized plasmid backbones
+(25ng/ul at 50ul) should be stored at 4C or lower</span></p>
+<p class=MsoListParagraph style='margin-left:36.0pt;text-indent:-36.0pt'><span
+lang=EN-US style='font-size:15.0pt;font-family:"Times New Roman","serif"'>1.2<span
+style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:15.0pt;font-family:"Times New Roman","serif"'>Usage</span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>1.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>With a pipette tip, punch a hole through
+the foil cover into the corresponding well to the Biobrick&#8482;-standard part that
+you want. </span><span lang=EN-US><a
+href="http://partsregistry.org/Help:Spring_2010_DNA_distribution#Distribution_plate_orientation"
+title="http://partsregistry.org/Help:Spring_2010_DNA_distribution#Distribution_plate_orientation"><span
+style='font-size:12.0pt;line-height:150%;font-family:"Times New Roman","serif";
+color:windowtext;text-decoration:none'>Make sure you have properly oriented the
+plate</span></a></span><span lang=EN-US style='font-size:12.0pt;line-height:
+%;font-family:"Times New Roman","serif"'>. We recommend that you do not
+remove the foil cover, as it could lead to cross contamination between the
+wells. </span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>2.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US><a
+href="http://partsregistry.org/Image:IGEM06DistPlateTop.jpg"
+title="&quot;Top view of plates containing dry DNA; red circle indicates well 13H&quot; "><span
+style='font-size:12.0pt;line-height:150%;font-family:"Times New Roman","serif";
+color:windowtext;text-decoration:none'><img border=0 width=200 height=134
+id="图片 9" src="/wiki/images/5/5d/Whu-Proto1.jpg"
+alt="说明: Top view of plates containing dry DNA; red circle indicates well 13H"></span></a></span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>3.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Add 10uL of diH2O (deionized water), the
+resuspension will become red due to the cresol red dye used during
+manufacturing. </span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>4.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Pipette 1 or 2uL of the resuspended DNA </span><span
+lang=EN-US><a href="http://partsregistry.org/Help:Transformation_Protocol"
+title="Help:Transformation Protocol"><span style='font-size:12.0pt;line-height:
+%;font-family:"Times New Roman","serif";color:windowtext;text-decoration:
+none'>transform</span></a></span><span lang=EN-US style='font-size:12.0pt;
+line-height:150%;font-family:"Times New Roman","serif"'> into your desired
+competent cells, plate bacteria with the appropriate antibiotic* and grow
+overnight. </span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>5.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Pick a single bacterial colony and
+transfer it into LB medium. Incubate the culture for 18 hours with vigorous
+agitation.</span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>6.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Store the single colony in physiological
+saline and on inclined plane, and make recognizable marks on the tube and on
+the notebook.</span></p>
+<a name="poc"><a href="#top" title="Back to top">
+<p class=MsoNormal style='line-height:150%'><span style='font-size:20.0pt;
+line-height:150%;font-family:宋体'>Ⅱ</span><span lang=EN-US style='font-size:
+.0pt;line-height:150%;font-family:"Times New Roman","serif"'>. Preparation of
+competent cells (Using Calcium Chloride)</span></p></a></a>
+<p class=MsoNormal><span lang=EN-US style='font-size:15.0pt;font-family:"Times New Roman","serif"'>2.1&nbsp;
+Day 0: </span></p>
+<p class=MsoNormal style='line-height:150%'><span lang=EN-US style='font-size:
+.0pt;line-height:150%;font-family:"Times New Roman","serif"'>&nbsp;&nbsp;&nbsp;
+</span><span lang=EN-US style='font-size:12.0pt;line-height:150%;font-family:
+"Times New Roman","serif"'>Pick a single bacterial colony from a plate that has
+been incubated for 16-20 hours at 37</span><span style='font-size:12.0pt;
+line-height:150%;font-family:宋体'>℃</span><span lang=EN-US style='font-size:
+.0pt;line-height:150%;font-family:"Times New Roman","serif"'>. Transfer the
+colony into LB medium. Incubate the culture overnight (about 16 hours) at 37</span><span
+style='font-size:12.0pt;line-height:150%;font-family:宋体'>℃</span><span
+lang=EN-US style='font-size:12.0pt;line-height:150%;font-family:"Times New Roman","serif"'>
+with vigorous shaking.</span></p>
+<p class=MsoNormal><span lang=EN-US style='font-size:15.0pt;font-family:"Times New Roman","serif"'>2.2&nbsp;
+Day 1: </span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>1.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Transfer 1 ml of the culture into 100 ml
+of LB medium. Incubate the culture for 2.5-3 hours at 37</span><span
+style='font-size:12.0pt;line-height:150%;font-family:宋体'>℃</span><span
+lang=EN-US style='font-size:12.0pt;line-height:150%;font-family:"Times New Roman","serif"'>
+with vigorous agitation (250-300rpm).</span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>2.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Transfer 1.5 ml of the culture into
+sterile ice-cold 1.5ml polypropylene tubes. Cool the cultures by storing the
+tubes on ice for 10 minutes.</span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>3.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Recover the cells by centrifugation at 2500
+rpm for 5minutes at 4</span><span style='font-size:12.0pt;line-height:150%;
+font-family:宋体'>℃</span><span lang=EN-US style='font-size:12.0pt;line-height:
+%;font-family:"Times New Roman","serif"'>.</span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>4.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Decant the medium from the cell pellets.
+Resuspend each pellet by swirling or gentle vortexing in 100ml of ice-cold 0.1M
+CaCl2 solution. Store the tubes on ice for 20minutes.</span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>5.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Recover the cells by centrifugation at
+rpm for 5 minutes at 4</span><span style='font-size:12.0pt;line-height:
+%;font-family:宋体'>℃</span><span lang=EN-US style='font-size:12.0pt;
+line-height:150%;font-family:"Times New Roman","serif"'>.</span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>6.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Decant the medium from the cell pellets.
+Resuspend each pellet by swirling or gentle vortexing in 100ml of ice-cold 0.1M
+CaCl2 solution.</span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>7.<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>The suspension of competent cells should
+be immediately used in transformation.</span></p>
+<p class=MsoNormal align=left style='margin-bottom:9.6pt;text-align:left'><b><span
+lang=EN-US style='font-size:12.0pt;font-family:"Times New Roman","serif"'>&nbsp;</span></b></p>
+<p class=MsoNormal align=left style='margin-bottom:9.6pt;text-align:left'><b><span
+lang=EN-US style='font-size:12.0pt;font-family:"Times New Roman","serif";
+color:red'>Attention:</span></b></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>[1]<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Mix gently </span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>[2]<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>The newly prepared competent cells
+should be transformed immediately. They cannot be stored for long (except in
+-80</span><span style='font-size:12.0pt;line-height:150%;font-family:宋体'>℃</span><span
+lang=EN-US style='font-size:12.0pt;line-height:150%;font-family:"Times New Roman","serif"'>)</span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>[3]<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Keep sterile environment during
+operation (sterilize the clean bench by ultra-violet, sterilize hands and implements
+by alcohol). </span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:-21.0pt;
+line-height:150%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>[4]<span style='font:7.0pt "Times New Roman"'>&nbsp;&nbsp;&nbsp;&nbsp;
+</span></span><span lang=EN-US style='font-size:12.0pt;line-height:150%;
+font-family:"Times New Roman","serif"'>Use heat-shock method to transform. </span></p>
+<p class=MsoListParagraph style='margin-left:21.0pt;text-indent:0cm;line-height:
+%'><span lang=EN-US style='font-size:12.0pt;line-height:150%;font-family:
+"Times New Roman","serif"'>&nbsp;</span></p>
 	</div>
 	<h3><a href="#">2rd Question</a></h3>