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Revision as of 10:31, 2 September 2015

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Project

  • 1. Overview

  • 2. Background

    • 2.1 Challenges
    • 2.2 Solution
  • 3. Design

  • 4. Protocol

  • 5. Summary and Result

  • 1. Overview

    Cells sense the environment, process information, and make response to stimuli. To make cells work well in complex natural environments, lots of processes have to be preset to react to various signals. However, when well-characterized modules are combined to construct higher order systems, unpredictable behaviors often occur because of the interplay between modules. Another significant problem is that complex integrated systems composed of numerous parts may cause cell overload.

    Figure 1. Schematic demonstration of HIV

    We proposed an elegant method to design higher order systems. Instead of merely combining different functional modules, we constructed one integrated processing module with fewer parts by utilizing the common structures between modules. The circuit we designed is a rewirable one and the topological structure of the processing module can be altered to adapt to environmental change. The basic idea is to rewire the connections between parts and devices to implement multiple functions with the help of the site-specific recombination systems.

    Our design approach may lead to a revolutionary step towards system integration in synthetic biology. Potential fields of application include organism development, living therapeutics and environment improvement.

    2. Background

    Since its inception more than a decade ago, synthetic biology has undergone considerable development and has attained significant achievements with the help of the engineering slant. However, there are still obstacles to build a cell. Engineers try to abstract the DNA sequences into some standard functional parts and assemble them using some principles in electrical engineering. So far, the limited understanding of biological system prevents us to combine parts and modules to create larger scale systems. The complexity of synthetic systems didn’t increase rapidly as the Moore’s law (Purnick and Weiss, 2009).

    2.1 Challenges

    There are some common problems that make the circuits we designed not work as our expected. Many failure modes have been collated by Brophy and Voigy in their review (Brophy and Voigt, 2014). In our project, we mainly focus on two modes, crosstalk and host overload, that emerge especially when we create more sophisticated systems. More specifically, regulators may interact with each other’s targets leading to errors in the desired operation, and the synthetic circuits may compete with natural parts that maintain the normal cellular processes for limited resources.

    2.2 Solution

    We designed a time-sharing system that can process information according to the input signal. Cells rewire its synthetic circuit to alter the topological structure of regulatory pathway when they receive the corresponding stimuli. In this way, we reuse the existing synthetic module rather than add a new one to implement another function, which reduces the resource cost in running unnecessary function and prevents the interplay between parallel modules. After overcoming these two big problems, our engineered cells are more versatile and flexible in information processing.

    3. Design

    Cells sense the environment, process information, and make response to stimuli. To make cells work well in complex natural environments, lots of processes have to be preset to react to various signals. However, when well-characterized modules are combined to construct higher order systems, unpredictable behaviors often occur because of the interplay between modules. Another significant problem is that complex integrated systems composed of numerous parts may cause cell overload.

    Figure 2. China Tongji logo

    Our design approach may lead to a revolutionary step towards system integration in synthetic biology. Potential fields of application include organism development, living therapeutics and environment improvement.

    4. Protocol

    4.1 Introduction

    Our project aims to control C.elegans’ movement by expressing chR2 in their muscle and neuron. In our plan, we will make over 20 parts of 3 kinds of channelrhodopsins with 5 different promoters.

    First of all, we need to design the PCR primers with primer 5.Then we run taq PCR or pfu PCR to get our parts out of the C.elegans’ genome or plasmids.After that, we do the digestion of gene parts and vector pPD95.77. Use traditional method to do the ligation and transformation. Besides, we also use seamless cloning to deal with some difficult ligations. The last step in molecular construction is plasmid extraction.

    Then we come to the C.elegans part, which includes microinjection, making NGM and ATR plates and seed plates. All the details will show below.

    4.2 Taq PCR

    (1) Put dNTP, primers, template, taqbuffer and taq enzyme on ice;

    (2) Prepare the mix liquid:

    Experimental MaterialDose
    Template1ul
    Primer-Front1ul
    Primer-Reverse1ul
    dNTPs4ul
    Taq PCR buffer5ul
    taq enzyme0.25ul
    ddH2O37.75ul
    Total volume50ul

    (3) Mix solution well;

    (4) Use the PCR machine and amplification the gene:

    MethodTime
    95℃ pre-denaturation10min
    95℃ denaturation30s35cycles
    60℃ anneal30s
    72℃ extend1min
    4℃ saveend

    4.3 Pfu PCR

    (1) Put dNTP, primers, template,pfubuffer andpfuenzyme on ice;

    (2) Prepare the mix liquid:

    Experimental MaterialDose
    Template1ul
    Primer-Front2.5ul
    Primer-Reverse2.5ul
    dNTPs5ul
    5*Loading Buffer10ul
    Pfu DNA polymerase1ul
    ddH2O27ul
    Total volume50ul

    (3) Mix solution well;

    (4) Use the PCR machine and amplification the gene:

    MethodTime
    95℃ pre-denaturation10min
    95℃ denaturation30s35cycles
    60℃ anneal30s
    72℃ extend1min
    4℃ saveend

    4.4 AGE ( agarose gel electrophoresis )

    (1) make of gel with 0.5g agarose and 50ml 10X TAE, add 2 drops of EB to dye the gel;

    (2) mix the PCR sample with 10x loading buffer;

    (3) 220V 30min;

    (4)use UV light to view the result.

    4.5 Gel extraction

    (1) Excise the agarose gel slice containing the DNA fragment of interest with a clean, sharp scalpel under ultraviolet illumination. Briefly place the excised gel slice on absorbent toweling to remove residual buffer. Transfer the gel slice to a piece or plastic wrap or a weighing boat. Mince the gel into small pieces and weigh. In this application, the weight of gel is regarded as equivalent to the volume. For example, 100 mg of gel is equivalent to a 100 μl volume. Transfer the gel slice into a 1.5 ml microfuge tube.

    (2) Add a 3x sample volume of Buffer DE-A.

    (3) Resuspend the gel in Buffer DE-A by vortexing. Heat at 75°C until the gel is completely dissolved (typically, 6-8 minutes) Heat at 40°C if low-melt agarose gel is used. Intermittent vortexing (every 2-3 minutes) will accelerate gel solubilization.

    (4) Add 0.5x Buffer DE-A volume of Buffer DE-B, mix. If the DNA fragment is less than 400 bp, supplement further with a 1x sample volume of isopropanol.

    Example: For a 1% gel slice equivalent to 100 μl, add the following:

    • 300 μl Buffer DE-A

    • 150 μl Buffer DE-B

    If the DNA fragment is < 400 bp, you would also add:

    • 100 μl of isopropanol.

    (5) Place a Miniprep column into a 2 ml microfuge tube (provided) Transfer the solubilized agarose from Step 4 into the column. Centrifuge at 12,000xg for 1 minute.

    (6) Discard the filtrate from the 2 ml microfuge tube. Return the Miniprep column to the 2 ml microfuge tube and add 500 μl of Buffer W1. Centrifuge at 12,000xg for 30 seconds.

    (7) Discard the filtrate from the 2 ml microfuge tube. Return the Miniprep column to the 2 ml microfuge tube and add 700 μl of Buffer W2. Centrifuge at 12,000xg for 30 seconds.

    (8) Discard the filtrate from the 2 ml microfuge tube. Place the Miniprep column back into the 2 ml microfuge tube. Add a second 700 μl aliquot of Buffer W2 and centrifuge at 12,000xg for 1 minute.

    (9) Discard the filtrate from the 2 ml microfuge tube. Place the Miniprep column back into the 2 ml microfuge tube. Centrifuge at 12,000xg for 1 minute.

    (10) Transfer the Miniprep column into a clean 1.5 ml microfuge tube (provided) To elute the DNA, add 25-30 μl of Eluent or deionized water to the center of the membrane. Let it stand for 1 minute at room temperature. Centrifuge at 12,000xg for 1 minute.

    4.6 Digestion & ligation

    4.6.1 Digestion

    (1)Add enzyme A 1ul and enzyme B 1ul;

    (2)Add plasmid 4ul or gene 10ul;

    (3)Add buffer 2ul;

    (4)Add enough water;

    (5)37℃ 2h;

    (6)Do agarose gel electrophoresis;

    (7)Gel extraction.

    4.6.2 Ligase reaction

    (1)Add 1ul ligase;

    (2)Add 2ul ligase buffer;

    (3)Add 10ul gene that have digested;

    (4)Add 3ul digested plasmid;

    (5)Add water;

    (6)12℃ 8h.

    4.7 Seamless cloning

    The design of primers of PCR amplification for cloning of your sequence of interest is based on the same principles as the design of PCR primers for any sequence. The only difference is that simply add the 14-18 bases of vector sequence to the 5’end of your sequence-specific PCR primers when designing primers. After PCR clean up, the resulting PCR- amplified insert is ready for Fast Seamless Cloning.

    (1) Digest the vector with two enzymes;

    (2) set up fast seamless gene cloning reaction: 7.5ul seamless cloning enzyme mix with 1ul linearizedvector and 1.5ul gene;

    (3) 42℃ 30min;

    (4) transformation.

    4.8 Transformation

    (1) Get competence E.coli from -80C fridge;

    (2) Add 15ul plasmid liquid into competence E.coli, put it in ice water for 15-30min. then give it a 42℃ heat shock for 90 sec. finally put it out of the 42℃ water bath as quick as possible. Put it into ice water for 5 min;

    (3) Add 500ul LB into competence E.coli;

    (4) At 37℃ we train them for 1h;

    (5) Add 100ul into a LB plate which has already added ampicillin. Put them in the 37C incubator for 14h-16h.

    4.9 Plasmid Extraction

    (1) Put the bacterium liquid in the EP tube, Centrifuge at 12100rpm for 1 minute at room temperature;

    (2) Pour out the supernatant as clean as possible;

    (3) Add 150 ul P1 to the bacteria sediment, suspend the bacteria in P1 buffer;

    (4) Add 150 ul P2, and shake the tube gentle 6-8 times until the liquid become in clear purple color;

    (5) Add 350 ul P5, and shake it quickly for 12-20 times;

    (6) Centrifuge at 12100rpm for 2 minutes at room temperature;

    (7) Transfer 700 ul of the mixture(from Step 6) into a clean DNA Mini Column assembled in a 2ml collection tube(provided) Centrifuge at 12100rpm for 2 min at room temperature to pass solution through column;

    (8) Pour out the liquid;

    (9) Add 300ul PWT in the column, Centrifuge at 12100rpm for 2 min at room temperature to pass solution through column;

    (10) Pour out the liquid and centrifuge again at 12100rpm for 1 min at room temperature;

    (11) Place column into a new clean 1.5ml micro-centrifuge tube. Add 50ul 50℃ ddH2O directly onto the column matrix and centrifuge at 12100rpm for 2min to elute DNA;

    (12) Exam the OD.

    4.10 Microinjection

    4.10.1 Equipment

    (1) Injection table;

    (2) Inverted DIC microscope;( Zeiss Observe.A1)

    (3) Micromanipulator;(Zeiss)

    (4) Pressurized injection system with needle holder;

    (5)Needle puller. Sutter instruments MODEL P-1000 micropipette pullers.

    4.10.2 Materials

    (1)Microinjection needles;

    (2)Injection pads.(Bring 2% agarose in water to a boil, mix well, and place in a heat block. Using a broken Pasteur pipette or a cut-off P200 tip, place a drop (~100ul) of hot agarose onto a #1, 50X22-mm glass coverslip. Quickly place a second coverslip on the drop and lightly tap it. Alternatively, place several drops on the first coverslip, which should merge and mostly cover the surface after adding the second coverslip;)

    (3) Injection oil. Series 700 Halocarbon oil;

    (4) Worm pick;

    (5) M9 buffer;

    (6)Worms; (Well-fed, young to middle-aged (≥1day old) gravid hermaphrodites with a full but single row of eggs.)

    (7)Needle-loading pipettes.

    4.10.3 Method

    (1) Fill a needle-loading pipette by capillary action with ≥ 1 ul of DNA injection mix;

    (2) Insert the pipette tip in through the back of the injection needle, and expel injection mix onto the needle's internal filament;

    (3) Place a loaded needle into the needle holder and mount on the manipulator;

    (4) Position the needle so that the tip is in the center of the microscope's field of view using the 5X objective;

    (5) Place a drop of oil on an injection pad and place under a dissecting microscope on top of a small Petri plate cover;

    (6) Scoop one to several worms from a bacteria-free region of an NGM plate with a naked pick and transfer to the oil drop. Avoid contact with the worm's head. Alternatively, first touch the worm pick to the oil, and use the oil droplet to pick up the animals from a bacteria-free region. The idea is to minimize transfer of bacteria to the pad;

    (7) Flame then cool the worm pick and use it to position the worms in the oil drop, and to gently push them down onto the pad. Orient the worms in rows with their ventral sides facing the same direction (opposite the needle direction) If the worms fail to adhere to the pad, move to a new location or rub the bodies with the pick to remove water or bacteria droplets. If adherence is still a problem re-bake the pads or use thicker or higher concentration agarose pads (see above)

    (8) Transfer the slide face-up onto the microscope stage. Center the first worm to be injected and focus using the 5X objective. Move the needle down and in close proximity to the dorsal surface of the first animal. Switch to the 40X objective and focus on the worm;

    (9) First make sure the needle is flowing;

    (10) Insert the needle into the worm;

    (11)Inject the DNA solution;

    (12) Recover the worms: (Return the coverslip to the dissecting scope, and add a drop (~20 ul) of recovery buffer on the worms.)

    4.10.4 Preparation of NGM plates

    Equipment and Reagents

    • NaCl

    • Agar

    • Peptone

    • 5 mg/ml cholesterol in ethanol (Do not autoclave!)

    • 1 M KPO4 buffer pH 6.0 (108.3 g KH2PO4, 35.6 g K2HPO4, H2O to 1 litre)

    • 1M MgSO4

    • Petri plates

    • Peristaltic pump

    5. Summary and Result

    Cells sense the environment, process information, and make response to stimuli. To make cells work well in complex natural environments, lots of processes have to be preset to react to various signals. However, when well-characterized modules are combined to construct higher order systems, unpredictable behaviors often occur because of the interplay between modules. Another significant problem is that complex integrated systems composed of numerous parts may cause cell overload.

    Figure 2. China_Tongji_iGEM_logo

    Our design approach may lead to a revolutionary step towards system integration in synthetic biology. Potential fields of application include organism development, living therapeutics and environment improvement.