Team:HKUST/Protocols/Transformation to Ecoli

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Revision as of 15:53, 19 October 2009

Salt and Soap template

Main Parts

Resources

a

Transformation to yeast

Purpose: To transform desired constructed plamid DNA to yeast to test its effect.

Materials: LiOAc solution, PEG4000 solution, DMSO (dimethyl sulfoxide), yeast strain, desired plasmid, YEPD, SD media with specific selection marker absent (-Leu, -His, or -Ura), ddH2O

Procedure:

a.A stationary culture of yeast grown in YEPD is used to inoculate 10mL of YEPD in a 100mL Pyrex flask.
b.Cells are grown at 30 °C with shaking (200 rpm) until a density of 1-4x107 is reached (OD660=0.4).
c.Yeast is transformed into 4 sterile 1.5mL tubes and are centrifuged for 2mins (4,000 rpm).
d.Damp off media and wash the pellet with 100μL ddH2O (to culture 1:1). Resuspend the cells by gently shake it or flip it.
e.Centrifuge it again for 2mins (4,000 rpm). Remove the supernatant.
f.Wash the pellet with 1mL LiOAc solution and pour it into a single tube. Resuspend the cell by gently shake it or flip it.
g.Repeat step e and f once.
h.Add 100μL of yeast suspension to a 1.5mL microcentrifuge tube, and add 10μL of DNA to be transformed. Mix them gently and stand the tube at room temperature for 5mins.
i.Add 280μL PEG4000 solution. Mix it gently by inverting 4-6 times, then the tube is stored at 30 °C for 45mins without shaking.
j.Add 43μL DMSO to give an approximate 10% (volume percentage) DMSO solution. Mix the solution gently by inverting.
k.Heat shock at 42°C for 5mins.
l.Centrifuge it for time long enough to get pellet (usually 5 sec) at 12,000rpm.
m.Remove the supernatant and wash it with ddH2O.
n.Centrifuge it again for 50sec (13,000 rpm). Remove the supernatant.
o.Resuspend the cell with 1mL ddH2O.
p.Plate the solution on SD media with specific selection marker absent.

Tips:

Ignite the fire for sterile environment when transforming the yeast cell, since there is no any antibiotic in the culture.br>

Safety tips:

Be careful with the fire, and extinguish it after use.

iGEM 2009

@@ Line 1: / Line 1: @@
-. Transformation to yeast
+<html xmlns="http://www.w3.org/1999/xhtml">
-   Purpose: To transform desired constructed plamid DNA to yeast to test its effect.
+<head>
-    Materials: LiOAc solution, PEG4000 solution, DMSO (dimethyl sulfoxide), yeast strain, desired plasmid, YEPD, SD media with specific selection marker absent (-Leu, -His, or -Ura), ddH2O
+<meta http-equiv="Content-Type" content="text/html; charset=iso-8859-1" />
-   Procedure:
+<link href="http://igem2009hkust.fileave.com/wiki/template/12092009/style.css " rel="stylesheet" type="text/css" />
-   a.A stationary culture of yeast grown in YEPD is used to inoculate 10mL of YEPD in a 100mL Pyrex flask.
+<title>Salt and Soap template</title>
-    b.Cells are grown at 30 °C with shaking (200 rpm) until a density of 1-4x107 is reached (OD660=0.4).
+</head>
-    c.Yeast is transformed into 4 sterile 1.5mL tubes and are centrifuged for 2mins (4,000 rpm).
-    d.Damp off media and wash the pellet with 100μL ddH2O (to culture 1:1). Resuspend the cells by gently shake it or flip it.
+<bodyxx>
-    e.Centrifuge it again for 2mins (4,000 rpm). Remove the supernatant.
+<div id="containerxx">
-    f.Wash the pellet with 1mL LiOAc solution and pour it into a single tube. Resuspend the cell by gently shake it or flip it.
+	<div id="headerxx">
-    g.Repeat step e and f once.
-    h.Add 100μL of yeast suspension to a 1.5mL microcentrifuge tube, and add 10μL of DNA to be transformed. Mix them gently and stand the tube at room temperature for 5mins.
+	</div>
-    i.Add 280μL PEG4000 solution. Mix it gently by inverting 4-6 times, then the tube is stored at 30 °C for 45mins without shaking.
+	<div id="borderxx">
-    j.Add 43μL DMSO to give an approximate 10% (volume percentage) DMSO solution. Mix the solution gently by inverting.
+		<div id="mainxx">
-    k.Heat shock at 42°C for 5mins.
+			<div id="leftxx">
-    l.Centrifuge it for time long enough to get pellet (usually 5 sec) at 12,000rpm.
+				<div id="menuxx">
-    m.Remove the supernatant and wash it with ddH2O.
+					<ul>
-    n.Centrifuge it again for 50sec (13,000 rpm). Remove the supernatant.
+<li><a href="https://2009.igem.org/Team:HKUST">Home</a></li>
-    o.Resuspend the cell with 1mL ddH2O.
+<li><a href="https://2009.igem.org/Team:HKUST/Team">Our Team</a></li>
-    p.Plate the solution on SD media with specific selection marker absent.
+<li><a href="https://2009.igem.org/Team:HKUST/Project">Project Description</a></li>
-   Tips:
-   •Ignite the fire for sterile environment when transforming the yeast cell, since there is no any antibiotic in the culture.
+<b>
-   Safety Tips:
+<span style="color:green">
-   •Be careful with the fire, and extinguish it after use.
+<li>Main Parts</li>
+</span>
+</b>
+<li><a href="https://2009.igem.org/Team:HKUST/OdorantSensoring">Odorant Sensoring</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/AttranctantProduction">Attranctant Production</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/ToxinProduction">Toxin Production</a></li>
+<b>
+<span style="color:green">
+<li>Resources</li>
+</span>
+</b>
+<li><a href="https://2009.igem.org/Team:HKUST/Lab Notebook">Lab Notebook</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Parts">Parts Submitted </a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols">Protocol List</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Resourses">Other Resources</a></li>
+					</ul>
+				</div>
+				<div id="menubottom">
+					<ul>
+<li><a href="https://2009.igem.org/Team:Gallery">Gallery</a></li>
+<li><a href="https://2009.igem.org/Team:Consolidation">Consolidation</a></li>
+<li><a href="https://2009.igem.org/Team:Acknowledgement">Acknowledgement</a></li>
+					</ul>
+				</div>
+			</div>
+			<div id="rightxx">
+		<div class="contentlist">					<h3>a</h3>
+</div>
+				<div class="contentxx">
+<p>Transformation to yeast</p>
+<p> Purpose: To transform desired constructed plamid DNA to yeast to test its effect. </p>
+    Materials: LiOAc solution, PEG4000 solution, DMSO (dimethyl sulfoxide), yeast strain, desired plasmid, YEPD, SD media with specific selection marker absent (-Leu, -His, or -Ura), ddH2O <br><br>
+<p>Procedure: </p>
+a.A stationary culture of yeast grown in YEPD is used to inoculate 10mL of YEPD in a 100mL Pyrex flask.<br>
+    b.Cells are grown at 30 °C with shaking (200 rpm) until a density of 1-4x107 is reached (OD660=0.4).<br>
+    c.Yeast is transformed into 4 sterile 1.5mL tubes and are centrifuged for 2mins (4,000 rpm).<br>
+    d.Damp off media and wash the pellet with 100μL ddH2O (to culture 1:1). Resuspend the cells by gently shake it or flip it.<br>
+    e.Centrifuge it again for 2mins (4,000 rpm). Remove the supernatant.<br>
+    f.Wash the pellet with 1mL LiOAc solution and pour it into a single tube. Resuspend the cell by gently shake it or flip it. <br>
+    g.Repeat step e and f once.<br>
+    h.Add 100μL of yeast suspension to a 1.5mL microcentrifuge tube, and add 10μL of DNA to be transformed. Mix them gently and stand the tube at room temperature for 5mins.<br>
+    i.Add 280μL PEG4000 solution. Mix it gently by inverting 4-6 times, then the tube is stored at 30 °C for 45mins without shaking.<br>
+    j.Add 43μL DMSO to give an approximate 10% (volume percentage) DMSO solution. Mix the solution gently by inverting.<br>
+    k.Heat shock at 42°C for 5mins.<br>
+    l.Centrifuge it for time long enough to get pellet (usually 5 sec) at 12,000rpm.<br>
+    m.Remove the supernatant and wash it with ddH2O.<br>
+    n.Centrifuge it again for 50sec (13,000 rpm). Remove the supernatant.<br>
+    o.Resuspend the cell with 1mL ddH2O.<br>
+    p.Plate the solution on SD media with specific selection marker absent.<br>
+<p> Tips: </p>
+Ignite the fire for sterile environment when transforming the yeast cell, since there is no any antibiotic in the culture.br>
+<p> Safety tips: </p>
+Be careful with the fire, and extinguish it after use.		<br> <br>
+<ul>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/Agarose_gel" >Agarose gel preparation and gel
+electrophoresis</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/PCR">PCR (Taq, Vent)</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/PCR_cleanup">PCR product clean-up</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/Enzyme_digestion"> Enzyme digestion (vector, insert)</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/plasmid_extraction"> Plasmid DNA extraction</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/gel_cut"> Gel cutting</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/gel_extraction"> Gel extraction</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/Ethanol_precipitation"> Ethanol precipitation</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/Ligation"> Ligation</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/Transformation_to_Ecoli"> Transformation to E.coli</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/Transformation_to_yeast">Transformation to
+yeast</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/Cell_lysis"> Cell lysis</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/Yeast_genomic_DNA_extraction"> Yeast genomic DNA
+extraction</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/Western_blotting"> Western blotting</a></li>
+<li><a href="https://2009.igem.org/Team:HKUST/Protocols/GFP_testing"> GFP testing</a></li>
+</ul>
+				</div>
+				<div class="productxx">
+										<div class="clear"></div>
+				</div>
+			</div>
+			<div class="clear"></div>
+		</div>
+	</div>
+	<div id="footerxx">
+		<div id="copyright">
+			<span> iGEM 2009 <br /> </span>
+		</div>
+		<div id="payment"><img src="http://igem2009hkust.fileave.com/wiki/template/12092009/images/HKUSTLogo.jpg" alt="HKUST" /></div>
+	</div>
+	<div id="footerend"></div>
+</div>
+</bodyxx>
+</html>