Difference between revisions of "Team:Arizona State/Experiments"

Set up the following reaction using the restriction endonuclease that has the lowest salt concentration in its recommended buffer (total reaction volume 50 µl).
Set up the following digest reaction on ice:

table, th, td { border: 1px solid black; border-collapse: collapse; }

Components	Volume (µL)
dH2O	25
10X Fast Digest Buffer + Green Dye	3
MRV Vector	10
BbsI	1
SpeI	1

Mix components by pipetting the reaction mixture up and down, or by "flicking" the reaction tube.
Quick ("touch") spin-down in a microcentrifuge. Do not vortex the reaction.
Incubate

Brianna Lopez

Mini-Prep Protocol

Harvest Cell :

• Pellet 1-5 mL of an overnight recombinant E. coli culture by centrifugation. -The optimal volume of culture to use depends upon the plasmid and culture density.

For best yields for E. coli grown in LB:
use 1-3 mL of culture for high copy plasmids
use 1-5 mL of culture for low copy plasmids
for best yields for E. coli grown in TB or 2X YT:
use only 1 mL of culture

1. Resuspend Cells (verify that appropriate volume RNase A solution was added to the Resuspension Solution

Completely resuspend the bacterial pellet with 200 µL of the Resuspension Solution.
Vortex or pipette up and down to thoroughly resuspend the cells until homogenous

2. Lyse Cells

Lyse the resuspended cells by adding 200 µL of the Lysis Solution
Mix the contents by gentle inversion (6-8 times) until the mixture becomes clear and viscous (Don’t vortex)
Do not allow the lysis reaction to exceed 5 minutes

3. Neutralize

Precipitate the cell debris by adding 350 µL of the Neutralization/Binding Solution
Gently invert the tube 4-6 times
Pellet the cell debris by centrifuging at ≥ 12,000 x g or maximum speed for 10 minutes
Cell debris, proteins, lipids, SDS, and chromosomal DNA should fall out as a cloudy, viscous precipitate.
If the supernatant contains a large amount of floating particulates after centrifugation, re-centrifuge the supernatant

4. Prepare Column

Insert a GenElute Miniprep Binding Column into a provided micro-centrifuge tube, if not already assembled
Add 500 µL of the Column Preparation Solution to each miniprep column and centrifuge at ≥ 12,000 x g for 30 seconds to 1 minute
Discard the flow-through liquid

5. Load cleared lysate

Transfer the cleared lysate from step 3 to the column prepared in step 4 and centrifuge at ≥ 12,000 x g for 30 seconds to 1 minute.
Discard the flow-through liquid

6. Wash Column (verify that ethanol has been added to the bottle of Wash Solution 2)

Add 750 µL of the diluted Wash Solution to the column
Centrifuge at ≥ 12,000 x g for 30 seconds to 1 minute
Discard the flow-through liquid and centrifuge again at maximum speed for 1-2 minutes without any additional Wash Solution to remove excess ethanol

7. Elute DNA

Transfer the column to a fresh collection tube. Add 100 µL of Elution Solution or molecular biology reagent water to the column
For DNA sequencing and other enzymatic application, use water or 5 Mm Tris-HCL, Ph 8.0, as an eluant
Centrifuge at ≥ 12,000 x g for 1 minute
Use immediately or store at -20˚C

Amber Mani

Growing samples in culture tubes for growth curves

This is used for growing up colony samples overnight for use in the plate reader.

Materials:

15ml culture tubes
LB (AMP or CHLOR)
Grown colonies ready to use on petri dishes
going to use micropipette to grab one colony at a time and add to LB in culture tubes

Procedure:

Collecting colonies and prepping the culture tubes

Best to do this in the evening so the cultures don't grow too long

Label each culture tube with the contents, date and your name
Add LB (AMP or CHLOR) to the culture tube. (general rule for how much LB - use about 1/4 the container volume. If tube is 15ml use about 3-4ml LB)
Take pipette and use a clean tip to collect ONE colony from the plate. Discard the tip INTO the culture tube with the colony on the tip.
Place the lid on the culture tube (not too tight so there is room for gas exchange)
Place the culture tubes into the shaking (37F) incubator for overnight growth.
In the morning you can use the Synergy plate reader to check the OD of the sample and dilute or add fresh LB as needed for the test you are running.

Making and running a gel

What you need and how much of it to make and run an agarose gel

Materials:

* 60 ml of TAE liquid into the flask for gel making.
* 0.6g of the agarose powder to the flask and swirled
* 6.0 μl of the Syber Safe DNA gel stain to the flask and swirled

Procedure:

How to make gel using ingredients

Gel making/running protocol used:

Started with adding 60 ml of TAE liquid into the flask for gel making.
Add 0.6g of the agarose powder to the flask and swirled
Use the microwave to heat the mixture (1 min, swirl and repeat) till all pieces dissolved and was a pure clear liquid
Add 6 μl of the Syber Safe DNA gel stain to the flask and swirled
Carefully poured the mixture into a blank gel tray with spacers in place.
Once the gel is cooled, add the KB+ DNA ladder to the first slot, 2nd slot is left blank and each following slot is to be loaded with 5 μl of each sample.
Once the slots are filled place the gel (still inside the plastic gel holder) into the Galileo/ BioRad electric current machine. Run for approximately 45 minutes at 110V.
To image the gel once finished, use the SynGene gel imager machine.

Chris Connot

Plate Induction & Imaging Protocol

Introduction

This protocol will lead you through the steps of setting up induction plates for Sender/Receiver combos as well as the imaging of the agar plate.

Materials

Agar plates
Sender/receiver bacteria on plates (suggested to be freshly transformed)
Positive/negative controls (GFP+/-Receiver)
MicroPipetter (05 ul to 200ul)
Pipette Tips
GeneSys Machine

o

Procedure

Induction Plate Setup

Procure agar plates and warm to 37℃.
Procure plates with desired bacteria (senders,receivers,positive/negative control)
design/print out template (fig. 1) for induction test

Fig 1: Induction Plate Layout

Using a micropipettor and a sterile tip, bend the tip on the back of the lid of the agar plate

Fig 2: Bent Tip Method

Use the bent tip to scrape bacteria from any of the required plates (sender/receiver, pos/neg controls)
Paint the bacteria (liberally) on the plate in the designated sections.
Be sure to add enough bacteria so that there is a semi-thick layer that is continuous throughout the designated area.

Imaging the Induction plates

Put magnetic cover on top of UV light ( will have to adjust placement after imaging)
Take off Lid of Culture plate

Fig 3: Prepping Culture Plate for imaging

Fig 4: SynGene Settings

Place culture plate on top of magnetic cover and close the tray. (Fig. 3)
Machine Settings: (Fig. 4)

Blots: Fluorescent Blot
Alexa 488
Epi Mid Wave UV
UV06

Press Green arrow once machine is done calibrating
Press Capture
Save as .sgd in order to have the original data still available to be able to save as .tif
If 3D imaging is needed:

click edit on the lower right side of the screen and click 3D on following screen (upper left)

If annotations are needed

proceed to the edit screen
click on annotate option in upper left hand corner
then place text over parts of the image you want to be annotated
save image in preferred format "as displayed" to save annotations.

Troubleshoot

Christina Smith

Xylaan Livingstone

What should this page contain?

Protocols
Experiments
Documentation of the development of your project

@@ Line 194: / Line 194: @@
 <h2> <ins>Chris Connot </ins></h2>
-<p> Insert here </p>
+<h2>Plate Induction & Imaging Protocol</h2>
+<h3>Introduction</h3>
+<p>This protocol will lead you through the steps of setting up induction plates for Sender/Receiver combos as well as the imaging of the agar plate. </p>
+<h3>Materials</h3>
+<ul>
+<li>Agar plates</li>
+<li>Sender/receiver bacteria on plates (suggested to be freshly transformed) </li>
+<li>Positive/negative controls (GFP+/-Receiver) </li>
+<li>MicroPipetter (05 ul to 200ul) </li>
+<li>Pipette Tips </li>
+<li>GeneSys Machine </li>
+</ul>
+o
+<h3>Procedure</h3>
+<b>Induction Plate Setup</b>
+<ol type="1">
+<li>Procure agar plates and warm to 37℃. </li>
+<li>Procure plates with desired bacteria (senders,receivers,positive/negative control)</li>
+<li>design/print out template (fig. 1) for induction test</li>
+<B>Fig 1: Induction Plate Layout</b>
+<img src=" https://static.igem.org/mediawiki/2017/8/8e/Inc_Pic_1.png"/>
+<li>Using a micropipettor and a sterile tip, bend the tip on the back of the lid of the agar plate </li>
+<b>Fig 2: Bent Tip Method</b>
+<img src=" https://static.igem.org/mediawiki/2017/8/8c/Inc_Pic_2.png"/>
+<li>Use the bent tip to scrape bacteria from any of the required plates (sender/receiver, pos/neg controls) </li>
+<li>Paint the bacteria (liberally) on the plate in the designated sections. </li>
+<li>Be sure to add enough bacteria so that there is a semi-thick layer that is continuous throughout the designated area. </li>
+<h3>Imaging the Induction plates </h3>
+<li>Put magnetic cover on top of UV light ( will have to adjust placement after imaging) </li>
+<li>Take off Lid of Culture plate </li>
+<img src=" https://static.igem.org/mediawiki/2017/f/ff/Inc_Pic_3.png"/>
+<b>Fig 3: Prepping Culture Plate for imaging </b>
+<img src=" https://static.igem.org/mediawiki/2017/2/26/Inc_pic_4.png"/>
+<b>Fig 4: SynGene Settings </b>
+<li>Place culture plate on top of magnetic cover and close the tray. (Fig. 3)</li>
+<li>Machine Settings: (Fig. 4) </li>
+<ul>
+<li>Blots: Fluorescent Blot</li>
+<li>Alexa 488</li>
+<li>Epi Mid Wave UV</li>
+<li>UV06</li>
+</ul>
+<li>Press Green arrow once machine is done calibrating</li>
+<li>Press Capture </li>
+<li>Save as .sgd in order to have the original data still available to be able to save as .tif </li>
+<li>If 3D imaging is needed: </li>
+<ul>
+<li>click edit on the lower right side of the screen and click 3D on following screen (upper left)</li>
+</ul>
+<Li>If annotations are needed</li>
+<ul>
+<li>proceed to the edit screen </li>
+<li>click on annotate option in upper left hand corner</li>
+<li>then place text over parts of the image you want to be annotated </li>
+<li>save image in preferred format "as displayed" to save annotations. </li>
+</ul>
+</ol>
 <h1> Troubleshoot </h1>

Difference between revisions of "Team:Arizona State/Experiments"

Revision as of 22:43, 28 September 2017

Arizona_State

Protocols

Christina Smith

Vector Digest Protocol for Modular Receiver Vector

Materials

Procedure

Brianna Lopez

Mini-Prep Protocol

Harvest Cell :

Amber Mani

Growing samples in culture tubes for growth curves

This is used for growing up colony samples overnight for use in the plate reader.

Procedure:

Collecting colonies and prepping the culture tubes

**Best to do this in the evening so the cultures don't grow too long**

Making and running a gel

What you need and how much of it to make and run an agarose gel

Materials:

Procedure:

How to make gel using ingredients

Gel making/running protocol used:

Chris Connot

Plate Induction & Imaging Protocol

Introduction

Materials

Procedure

Imaging the Induction plates

Troubleshoot

Christina Smith

Xylaan Livingstone

What should this page contain?

Inspiration

Best to do this in the evening so the cultures don't grow too long