Team:MIT mmethods
From 2010.igem.org
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<ul id="procedure"> | <ul id="procedure"> | ||
<li>a. Fill the devices with PDL (~100-150µL/device)</li> | <li>a. Fill the devices with PDL (~100-150µL/device)</li> | ||
- | <li>b. Wash twice with water after 24 hours. Make sure that all regions are washed, in order to avoid heterogeneous surface coating. If you get bubbles, try to remove them by using the pipette applying suction. </li></ul><br><br> | + | <li>b. Wash twice with water after 24 hours. Make sure that all regions are washed, in order to avoid heterogeneous surface coating. If you get bubbles, try to remove them by using the pipette applying suction. </li></ul> |
+ | <br><br> | ||
+ | <b class="bolded">Collagen Filling</b><br> | ||
+ | <ul id="procedure"> | ||
+ | Material<br> | ||
+ | <ul id="procedure"> | ||
+ | <li>a) PDL-coated microfluidic devices (e.g., 6)</li> | ||
+ | <li>b) Collagen Gel</li> | ||
+ | <li>c) Complete Medium</li></ul> | ||
+ | <br> | ||
+ | Procedure<br> | ||
+ | <ul id="procedure"> | ||
+ | <li>After PDL coating/drying, let the devices cool down for 30mins-1 hour at room temperature</li> | ||
+ | <li>1. Prepare collagen gel.</li> | ||
+ | <li>2. Draw 30µL of gel with the 200µL pipetter. Fill device from gel filling port. Fill gel most of the way from one port, but not all the way to the other gel filling port. Then, fill from the other port until gel interfaces merge. This will leave an inconsistent gel interface, but we do not have an option at this point.</li> | ||
+ | <li>3. Place each gel-filled device with the PDMS side facing up in the humidity box after it has been filled to avoid dryout.</li> | ||
+ | <li>4. Leave all devices for 1 hour in the incubator (in the humidity box) for the gel to polymerize</li> | ||
+ | <li>5. [IMPORTANT. This protocol establishes a stable pocket of air between the two medium channels at the outlet port.] Fill channels with medium from reservoir ports (~50-100µL). Gently fill medium until the channels have been filled to the cell seeding filling ports. Do NOT fill all the way to the outlet port. Instead, be sure to leave air at the channel intersection and in the outlet port. Place a droplet of medium over the outlet port to trap the air inside. Place devices in incubator. They will be ready for cell seeding in 24hours. </li></ul> | ||
</td> | </td> |
Revision as of 03:22, 15 October 2010
Bacterial Construction Protocol
Bacterial Experimental Protocol
Phage western blot
Mammalian Protocol
Microfluidic stress
Materials
mammalian protocol |
The Mammalian team focused on creating a pressure-sensitive promoter and creating a standard protocol for mammalian genes.
1 HTD Preparation Protocol 1.1 PDMS Mixture Preparation 1.2 PDMS Pouring 1.3 PDMS Baking 1.4 PDMS-Device punching and Bonding 1.5 PDMS Device Bonding 1.6 PDL coating 1.7 Collagen filling 1.8 Cell Seeding 2 Protocol for Deflection Experiments 2.1 Tubing Setup Details 2.2 Adding Medium to Channels 2.3 Connecting device to pressure valve 2.4 Microcontroller details |
HTD Preparation Protocols (adapted from Yannis, Alisha) PDMS Mixture Preparation Materials
Procedure
PDMS Pouring
PDMS Baking
PDMS-Device punching and Bonding
PDMS Device Bonding - Plasma Treatment
PDL Coating
Collagen Filling
Procedure |