Starter Kit Instructions
38 Pages
Preview
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BioLogic Chromatography System Starter Kit Instructions for the First Time User of the BioLogic Duo-Flow and BioLogic HR Systems Catalog Number 750-0135
For Technical Service Call Your Local Bio-Rad Office or in the U.S. Call 1-800-4BIORAD (1-800-424-6723)
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Table of Contents Introduction ...1 1. 2.
Starter Kit Components ...1 Other Materials You Will Need ...2
Part 1 BioLogic Duo-Flow Chromatography System Section 1
Preparation for Use of the System ...3
Section 2
Anion Exchange Separation of Protein Standards ...7
2.1 2.2 2.3 2.4 2.5
Overview of the Procedure ...7 Buffer Preparation ...8 Sample Preparation...8 Installation of the UNO™ Q1 column...8 Priming the Gradient Pumps and Equilibrating the UNO Q1 Column...9 Creating a Method ...9
2.6
Part 2 BioLogic HR Chromatography System Section 3
Preparation for Use of the System ...16
Section 4
Anion Exchange Separation of Protein Standards ...22
4.1 4.2 4.3 4.4 4.5
Overview of the Procedure ...22 Buffer Preparation ...23 Sample Preparation...23 Installation of the UNO Q1 Column...23 Priming the Gradient Pumps and Equilibrating the UNO Q1 Column...24 Creating a Method for the Manual BioLogic HR System...24 Creating a Method for the Automated BioLogic HR system ...31
4.6 4.7
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Introduction This instruction manual and starter kit contents may be used for both the BioLogic Duo-Flow and BioLogic HR Chromatography Systems. To use the starter kit with the BioLogic Duo-Flow System, refer to Section 1. To use the starter kit with the BioLogic HR System, refer to Section 3.
1. Starter Kit Components This starter kit contains the following items for running a separation. •
50 ml of buffer A, 250 mM Tris buffer pH 8.1 (10x concentrate)
•
50 ml of buffer B, 250 mM Tris buffer pH 8.1 plus 5.0 M NaCl (10x concentrate)
•
One vial of anion exchange protein standards (catalog number 125-0561)
•
One 1 ml disposable sample injection syringe
•
One 50 µl sample loop
•
One UNO Q1 column (catalog number 720-0001)
The chromatographic separation for this kit requires approximately 6 minutes.
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2. Other Materials You Will Need •
Filtered high quality water (i.e., HPLC grade water)
•
One 500 ml graduated cylinder
•
One 1 L sidearm flask
•
Stir bar and stir plate
•
Vacuum source for degassing
•
Two 500 ml bottles
•
Fraction collection tubes, 13 x 100 mm (at least 14 tubes)
•
100 ml beaker
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Section 1 Preparation for Use of the Duo-Flow System When the BioLogic Duo-Flow System is turned on, the Manual Control Screen is displayed. (see Figure 1) This screen consists of a series of boxes containing instrument faceplates which provide direct control of the gradient pumps, a fraction collector, the UV and conductivity detector range settings and valves. 1. Priming the BioLogic Duo-Flow Gradient Pumps. a. Immerse the gradient pump A and B inlet lines in a container of HPLC grade (filtered, degassed) or other high quality water. b. Connect the syringe (supplied with the fittings kit) to the priming port of pump head A. c. Turn the priming port counter-clockwise to open the seal. Gently withdraw the syringe plunger to draw water into the pump head. d. Repeat this operation several times until no air bubbles are visible in the inlet tubing. e. Tighten the priming port by turning it clockwise. f.
Repeat this priming procedure for pump head B.
2. Moving the Inject Valve to Purge Position. To change the status of an automated inject valve AVR7-3, go to the Manual Screen displayed on the controller monitor. If you plugged an inject valve into port 4, you will see a valve box designated AVR7-3 at port 4. The three radio buttons of this box correspond to valve positions as follows: L = Load position, I = Inject position, P = Purge position. To move the AVR7-3 valve to Purge position, click button P. Note: The default position at power up and at the end of a programmed method for the AVR7-3 is L. For all other automated valves the default is position 1.
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3. Purging the BioLogic Duo-Flow Pumps. a. Make sure that the inject valve is in the Purge position. b. Press the Purge buttons A and B on the front of the workstation. The gradient pumps will run and the indicator lights will flash green. c. Run both pumps for 2 minutes and then press the purge buttons again to stop the pump. BioLogic Duo-Flow - Default - no method File View Utilities Options Window New
Run
1 2
Browser Report
Gradient pump: F-10
Inlet B: High limit: Low limit:
wash load
Manual Setup Protocol
Run
Notes PostRun
Log
ON
UV Detector
Fraction Collector
Zero Baseline
System Local ml/min Mode: Rack: Rack 1 (128 tubes)
Flow rate: 1.00 Inlet A:
Help
New
Edit
Method Method
ON
OFF
%
100 0
%
1000
psi
0
psi
Start Tube:
1
End Tube:
128
Fraction size:
1.00
Tube number:
1
Chart Recorder Conductivity 500 range(mS/cm): ml
UV range (AU):
Volume left:
ON
Advance
Set
0.1 Event mark OFF
Signal Import Module START
STOP
START
STOP SIM 1 and SIM 2 connected
SVT3-2 at port 1
SV5-4 at port 2
AVR7-3 at port 4
AVR9-8 at port 5
I 1 1
2
L 4
I
2
3
P
8
2
6
4
7
3
5
Gradient Pump: F-10 0 %B 438 psi Flowrate of the gradient pump
0.00 ml/min
Conductivity 47.5 mS/cm
UV -0.00181 AU
SIM1/SIG 0.089 Volt
SIM2/pH 7.00 pH
Fig. 1. Manual Control Screen.
4. Control of the BioLogic Duo-Flow Pumps. The gradient pump parameters are set from the Manual Screen either by clicking in the appropriate field and entering a value from the keyboard or by using the spin arrows. You can set the flow rate between 0.1 to 10 ml/min and the gradient composition between 0% and 100% B. To start the pump, click the Start button. Note the running man icon. To change the pump parameters while the pump is running, enter the new value and then click on the set button.
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Pressure limits can be adjusted to match the pressure limits of a column. If the pressure limit is exceeded, the pump will stop and an alarm will sound. For now, set the high limit to 700 psi and the low limit to 20 psi. 5. Flushing the System through to the fraction collector. With the gradient pumps stopped, move the inject valve back to position L (Load) by clicking radio button L (AVR7-3) on the Manual Screen. Using the Manual Screen, set the pump flow rate at 1.0 ml/min and start the pump. Water will flow through the UV and conductivity flow cells and to the fraction collector, as described below. Using a Model 2128 Fraction Collector Connect the Model 2128 Fraction Collector by inserting the gray bus cable between it and the workstation. When it is connected, it will appear in the Manual Screen, as shown in Figure 2. BioLogic Duo-Flow - Default - no method File View Utilities Options Window New
Run
1 2
Browser Report
Gradient pump: F-10
Inlet B: High limit: Low limit:
wash load
Manual Setup Protocol
Run
Notes PostRun
Log
ON
UV Detector
Fraction Collector
Zero Baseline
System Local ml/min Mode: Rack: Rack 1 (128 tubes)
Flow rate: 1.00 Inlet A:
Help
New
Edit
Method Method
ON
OFF
%
100 0
%
1000
psi
0
psi
Start Tube:
1
End Tube:
128
Fraction size:
1.00
Tube number:
1
Chart Recorder Conductivity range(mS/cm): 500 ml
UV range (AU):
ON
Advance
Set
0.1 Event mark
Volume left:
OFF
Signal Import Module START
STOP
START
STOP SIM 1 and SIM 2 connected
SVT3-2 at port 1
SV5-4 at port 2
AVR7-3 at port 4
AVR9-8 at port 5
I 1 1
2
L 4
I
2
3
P
8
2
6
4
7
3
5
Gradient Pump: F-10 0 %B 438 psi Flowrate of the gradient pump
0.00 ml/min
UV -0.00181 AU
Conductivity
SIM1/SIG
SIM2/pH
47.5 mS/cm
0.089 Volt
7.00 pH
Fig. 2. Manual Control Screen showing Model 2128 Fraction Collector.
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The Model 2128 Fraction Collector has two operating modes. •
System: Controlled by the BioLogic Duo-Flow System.
•
Local: Controlled from its own faceplate.
For now, insure that the system button is selected. When in System mode, the fraction collector operates as follows. •
Control of the Model 2128 is identical whether or not the optional on-arm diverter valve is used. Without a valve, the drop-head returns to the waste trough during divert operations.
•
The fraction collector box on the Manual Screen will show fields for Rack type, Start tube, End tube, Fraction size–ml, Tube number, Volume left, a toggle button for Start and Stop and a button for Advance (see Figure 2).
6. Turning on the UV lamp. a. The UV lamp automatically turns on when you turn on power to the workstation. (The UV lamp is turned off and on by clicking the On and Off buttons in the Manual Screen (see Figure 2). You should now check that the lamp is on; the mercury lamp requires approximately 30 minutes to warm up. b. Clicking the Zero Baseline button will zero the UV signal. 7. The Manual Control Screen Chromatogram Window. A feature of the Manual Screen is the ability to display a chromatogram window showing UV and conductivity values over a 10 minute interval. This is useful during column equilibration. •
To access this feature, simply click the Chromatogram Window On button, at the far right of the toolbar (See Figure 2). The chromatogram window will be displayed at the bottom of the screen, over the valve position indicators. The time axis is reset automatically at the end of 10 minutes or reset manually by clicking the Clear Traces button. Use the scroll bars to change the scaling of the axes.
•
To close the Chromatogram Window, again click the toolbar button. The valve status indicators will reappear.
8. The Status Bar. At the bottom of the Manual Screen is a status bar which is continually updated with system parameters.
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Section 2 Anion Exchange Separation of Protein Standards The starter kit allows you to learn how to use the BioLogic Duo-Flow System by programming and running a separation of a premixed anion exchange standard containing equine myoglobin, conalbumin, chicken ovalbumin and soybean trypsin inhibitor, using a 1.3 ml UNO Q1 Column*. Equine myoglobin is not retained on the UNO Q1 Column and elutes in the void volume. Conalbumin, chicken ovalbumin and soybean trypsin inhibitor bind to the column and require increased salt concentrations for elution. Separation requires approximately 6 minutes.
2.1 Overview of the Procedure Run Conditions •
Buffer A = 25 mM Tris-HCl, pH 8.1
•
Buffer B = 25 mM Tris-HCl, pH 8.1, 0.5M NaCl
•
Flow rate
•
Sample volume 50 µl
•
UV detection
0.1 AUFS
•
Conductivity
100 mS/cm
4.00 ml/min
General Procedure Step 1
Buffer preparation
Step 2
Sample preparation
Step 3
Installation of the UNO Q1 column
Step 4
Priming the gradient pumps and equilibrating the column
Step 5
Writing a method a) Programming the Setup Editor b) Programming the Protocol Editor c) The Run Control Screen d) Starting a Run
* UNO Q1 Column: catalog number 720-0001
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2.2 Buffer Preparation Buffer A 1. Empty the contents of the bottle labeled buffer A into a 500 ml graduated cylinder and add filtered, high-quality water to 500 ml volume. 2. Place the contents of the graduated cylinder into a 1 L side-arm flask and drop in a stir bar. Cap the side arm flask, place it on a stir plate and connect it to a vacuum source. Degas the buffer for approximately 15 minutes with gentle stirring. 3
When degassing is complete, pour the buffer into a bottle and label appropriately.
Buffer B Prepare buffer B by following the same procedure for preparation of buffer A.
2.3 Sample Preparation 1. Remove the aluminum cap from the anion exchange standards vial. Slowly remove the rubber plug from the standards vial (the contents may be under vacuum). 2. Add 1.0 ml of prepared buffer A to the vial. 3. Replace the rubber stopper and gently invert the vial to solubilize the protein standards.
2.4 Installation of the UNO Q1 column Remove end caps from the UNO Q1 column. Keeping tubing lengths to a minimum, connect 1/16" tubing from port 4 of the inject valve to the column inlet. Connect the column outlet to the bottom of the UV flow cell. Secure the column in a vertical position.
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2.5 Priming the Gradient Pumps and Equilibrating the UNO Q1 Column Be sure the gradient pumps are stopped and the inject valve is in the purge position. Re-prime and purge pumps A and B as described in Section 2, step 1 of this manual. Set the inject valve to position L (Load). Set the flow rate to 2.0 ml/min. Set the UV range to 0.1 AUFS and the conductivity range to 100 mS/cm. 1. Wash the column with 6.5 ml (5 column volumes) of buffer B at 2 ml/min to remove the column storage solution. 2. Equilibrate the column with13 ml (10 column volumes) of 100% buffer A. The conductivity monitor on the status bar should now read approximately 3 mS/cm.
2.6 Creating a Method From the Manual Control screen, click the New Method toolbar button. You will see a dialog box asking for a method name (input Starter Kit Separation–Auto). Use the keyboard tab key to go to the Method Description and Method Author fields. Make an entry in these fields if desired and click the OK button. You will now see the Setup Editor. Programming the Setup Editor This information entered in the Setup Editor is important for the subsequent separation method. The buttons grouped in the left hand box (Available Devices) shows all the devices that could theoretically be connected to the BioLogic Duo-Flow System. The list of items in the right hand box (Devices in Setup) identifies those devices you wish to use in the subsequent method. The initial default Devices in Setup are a UV detector and a conductivity monitor as these come as standard with the BioLogic Duo-Flow System. The default devices in Setup can be changed by choosing Save setup as default from the Data pull-down menu.
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1. Click on the Fraction Collector button in the Available Devices box. A dialog box will appear asking you to choose the type of collector i.e. a generic collector, a Model 2110 or a Model 2128. Click on Model 2128 and click the OK button. You will see 2128 Fraction Collector in the Devices in Setup box. 2. Next, click on the AVR7-3 Valve button in the Available Devices box. You will see a dialog box with a pull-down menu under Valve Name/Function. You should see Sample Inject already selected. Other functions are available from the pull-down menu. This action is called valve function aliasing. You will see that the valve position names are Load for position 1, Inject for position 2, and Purge for position 3. BioLogic Duo-Flow - Jennifer - System training - Starter Kit File Edit View Utilities Options Window Help New
Edit
1 2
New
Method Method
Run
Browser Report
wash load
Manual Setup Protocol
Run
Notes PostRun
Log
Delete
Devices in setup
Available Devices
2128 Fraction Collector Aux Load Pump
Fraction Collector
UV Detector
Conductivity Monitor
UV Detector Conductivity Monitor SVT3-2 Valve - Fraction Collector Diverter
SIM1 1 pH
1
SVT3-2 Valve
AVR7-3 Valve
SIM1 Signal
SIM2 2 pH
2
SIM2 Signal
SV5-4 Valve
SV3
P U M P
Port 1
AVR9-8 Valve
INJECT
Gradient Pump: F-10 Inlet A:
25 mM Tris
Inlet B:
25 mM Tris + 0.5 M NaCl
Gradient Pump: F-10
UV
Conductivity
0 %B
-0.00284 AU
59.0 mS/cm
0.00ml/min
438 psi
SIM1/SIG 0.004 Volt
SIM1/pH 7.00 pH
Fig. 3. Setup editor.
3. Next, go to the box labeled Gradient Pump. Use the tab key or click and drag on the field buffer A to highlight it and type in 25 mM Tris, pH 8.1. Use the tab key to highlight buffer B and type 25 mM Tris + 0.5 M NaCl, pH 8.1. This operation is called aliasing the gradient pump inlets.
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4. The Setup Editor is now complete and you are now ready to program the separation steps. To see the protocol editor, click on the Protocol Editor toolbar menu button. Programming the Protocol Editor 1. From the Options pull-down menu, insure that Use Volume (ml) is selected, so that the programming base is Volume. BioLogic Duo-Flow - Dr. J. Smith - Starter Kit - UNO Q1 Edit View Utilities Options Window Help File Edit
New
1 2
New
Method Method Add Step
Run
Browser Report
wash load
Manual Setup Protocol
Volumn
Description
Run
Notes PostRun
1
0.0
Collect Fractions of size 2.00 ml during entire run
Load/Inject Sample
2
0.0
Chart Recorder
Linear Gradient
3
0.0
Isocratic Flow
Change Valve
4
1.0
Set Zero Baseline
5
1.0
Load/Inject Sample
Hold Alarm Zero Baseline
100%
Volume: 1.0 ml
0%
Flow: 4.00 ml/min
Isocratic Flow
Static Loop
Manual Inject Valve
Flow: 4.00 ml/min
25mM tris
100%
Volume: 0.8 ml
0% 100% --> 50% 0% --> 50% 0%
Flow: 4.00 ml/min Volume: 13.0 ml Flow: 4.00 ml/min Volume: 2.8 ml
100%
Flow: 4.00 ml/min
100%
Volume: 8.0 ml
0%
Flow: 4.00 ml/min
7
Linear Gradient
8
15.3
Isocratic Flow
25mM tris 25mM tris, 0.5M NaCl,
9
18.1
Isocratic Flow
25mM tris 25mM tris, 0.5M NaCl,
Gradient Pump: F-10 0 %B 1 psi Enter volume of sample to load
UV 0.00375 AU
Delete
UV Detector Load: Sample
25mM tris, 0.5M NaCl, 25mM tris 25mM tris, 0.5M NaCl,
UV Lamp
Repeat Steps
Paste
25mM tris, 0.5M NaCl,
2.3
End of Protocol
Copy
25mM tris
1.5
26.1
Cut
Turn ON
6
Chart Recorder
Log
Parameters
Isocratic Flow
Volume: 0.5 ml
Fraction Collection
0.00ml/min
Conductivity 3.59 mS/cm
SIM1/SIG -0.003 Volt
SIM1/pH
Fig. 4. Protocol editor.
2. Program the separation method listed below and in Figure 4. •
From the left side of the screen, press the Fraction collection button. In the pop-up window that appears, choose Collect All with a fraction size of 2.00 ml and a delay of 0. Make sure that you choose the correct rack number for the rack you will be using with the Model 2128.
•
Program the remaining steps using the add step icons from the left-hand side of the screen.
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Step Start Number (ml) 1. 2.
0.0 0.0
3. 4.
1.0 1.0
5.
1.5
6.
2.3
7.
15.3
8.
18.1
9.
26.1
Page 12
Step Collect fractions of size 2.00 ml during entire run Isocratic flow with 100% 25 mM tris, pH 8.1, 0% 25 mM tris, 0.5 M NaCl, pH 8.1 at 4.00 ml/min for 1.0 ml Set UV baseline to 0.0 Static loop: Inject 0.5 ml sample at 4.00 ml/min for 0.1 min Isocratic flow with 100% 25 mM tris, pH 8.1, 0% 25 mM tris, 0.5 M NaCl, pH 8.1 at 4.00 ml/min for 0.8 ml Linear gradient with 0% to 50% 25 mM tris, 0.5 M NaCl, pH 8.1 at 4.00 ml/min for 13.0 ml Isocratic flow with 0% 25 mM tris, pH 8.1, 100% 25 mM tris, 0.5 M NaCl, pH 8.1 at 4.00 ml/min for 2.8 ml Isocratic flow with 100% 25 mM tris, pH 8.1, 0% 25 mM tris, 0.5 M NaCl, pH 8.1 at 4.00 ml/min for 8.0 ml End of protocol
3. When you have finished programming the Protocol Editor, click on the toolbar button RUN. You will see a dialog box asking you to name the run. For now, type in Run 1 and click the OK button. You will now see the Run Control Screen (see Figure 5).
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The Run Control Screen 1. Use the toolbar buttons at the left-hand side of the screen to check that the screen display ranges for UV (0.1 AUFS) and conductivity (100 mS/cm) are correctly set and that the gradient pump pressure limits are appropriate (set to 700 psi High and 20 psi Low). 2. If you were equilibrating the column while writing the method, you will notice that the Status Bar is displaying the flow-rate and values for UV and conductivity. If necessary, you may wish to zero the UV trace by clicking on the Zero baseline button. This button may be clicked at any time. 3. To scale the on-screen chromatogram display axes, use the scroll bars located on the left and right axes of the chromatogram window. Starting the Run 1. Insure that sufficient tubes are in the fraction collector rack (approximately 14). The drophead will automatically move to tube 1 when the Run is started. 2. Insure that the AVR7-3 valve is in the LOAD position (position L). If it is not, return to the Manual Screen by clicking the toolbar Manual button and click on valve position L.
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BioLogic Duo-Flow - Carole Smith - Uno Q1 data - Uno Q1 - Standards Window File View Utilities Options Help New
Edit
Method Method Frac. Collector
Advance
1 2
New
Run
Browser Report
wash load
Manual Setup Protocol
Run
Notes PostRun
FullView
Log
UV
Conductivity
0.100
1
2
3
4
5
Fractions 6 7
8
9
10
11
12
13 50.0
100% Buffer B
Divert Valve 0.090
45.0
Waste
0.080
40.0
Grad. Pump High psi
0.070
35.0
Collect
1000 Low psi 0
0.060
Set
0.040
20.0
0.030
15.0
0.01 Cond Range
0.020
10.0
500
0.010
5.0
Event mark
0.000
Chart Recorder UV Range
0.050
30.0 25.0
50.0
0.0 -5.0
-0.010
UV Detector Zero Baseline Run Time 0:00.0
AU
00:00:00
00:02:00
00:04:00 Hr:Min:Sec
00:06:00 mS/cm
Protocol: > 1 0:00.0 Isocratic Flow with 100% Buffer B at 1.00 ml/min for 25.0 min Run Volume 0.0 ml
Gradient Pump: F-10 0.00ml/min 0 %B 0 psi
StepTime Left 0:24.9
Fraction Vol. Left
Valve Info
UV 0.00003 AU
Conductivity -0.014 mS/cm
SIM1/SIG
SIM1/pH
Fig. 5. Run control screen.
3. Insure that the 50 µl sample loop is connected to ports 3 and 6 of the inject valve. Completely fill the loop with sample protein standard via port 5 and a syringe and needle. Do not remove the syringe from the injection port after filling the loop or the sample will siphon to waste. 4. To launch the Run, click on the green Start toolbar button. The sample will be loaded automatically. 5. Clicking the Hold toolbar button will hold the gradient pumps at the current %B value and will not advance the programmed method until the Continue toolbar button is pressed. Clicking the Pause toolbar button will stop the pumps completely. Clicking the Continue toolbar button will re-start the pumps at exactly the point where the program was paused. 6. When this run is finished, the pumps automatically stop and a run finished message appears in the bottom right of the status bar. 7. Figure 5 shows a typical run screen and chromatogram for this separation.
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Section 3 Preparation for Use of the BioLogic HR System The procedures in this document are written for two configurations, which are distinguished by the following. •
Manual: Uses a V7-3 Manual Inject Valve, a Model 2110 Fraction Collector, and an SV3-2 Diverter Valve.
•
Automated: Uses an AV7-3 Automatic Inject Valve and a Model 2128 Fraction Collector.
When you turn on the BioLogic HR System, the Manual Control Screen is displayed (see Figure 6). This screen consists of a series of boxes containing instrument faceplates which provide direct control of the gradient pumps, a fraction collector, a chart recorder (apart from chart speed, which is set on the recorder itself), the UV and conductivity detector range settings and solenoid and automated valves. 1. Priming the BioLogic HR Gradient Pumps. a. Immerse the gradient pump A and B inlet lines in a container of HPLC grade (filtered, degassed) or other high quality water. b. Connect the syringe (supplied with the fittings kit) to the priming port of pump head A. c. Turn the priming port counter-clockwise to open the seal. Gently withdraw the syringe plunger to draw water into the pump head. d. Repeat this operation several times until no air bubbles are visible in the inlet tubing. e. Tighten the priming port by turning it clockwise. f.
Repeat this priming procedure for pump head B.
2. Moving the Inject Valve to Purge Position. •
For a manual inject valve V7-3, move the arm to the Purge position (left, then up, then left). The figure in the valve position window displays P. Flow from the gradient pumps will now go directly to waste, bypassing any column or detector downstream of the valve.
•
To change the status of an automated inject valve AV7-3, go to the Manual Screen displayed on the controller monitor.
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If you plugged an inject valve into port 4, you will see a valve box designated AV7-3 at port 4. The three radio buttons of this box correspond to valve positions as follows: L = Load position, I = Inject position, P = Purge position. To move the AV7-3 valve to Purge position, click button P. Note: The default position at power up and at the end of a programmed method for the AV7-3 is L and for all other automated valves is position 1. 3. Purging the BioLogic HR Pumps. With the inject valve in position P (Purge): a. Press the Purge buttons A and B on the front of the Workstation. The gradient pumps will run and the indicator lights will flash green. The default purge flow rate is 7 ml/min per pumphead, although this may be changed using the options (manual setup) pull-down menu. b. Run both pumps for 2 minutes and then press the Purge buttons again to stop the pump. BioLogicHR - Dr. J. Smith - Starter Kit - UNO Q1 File View Utilities Options Window New
Help 1 2
New
Edit
Method Method
Run
Browser Report
Fraction Collector
Gradient pump Flow rate: 4.00
wash load
Manual Setup Protocol
Run
Notes PostRun
Inlet B: High limit: Low limit:
ON
Zero Baseline
ml/min
ON Inlet A:
Log
UV Detector
OFF
%
100 0
%
1000
psi psi
0
Chart Recorder Conductivity range(mS/cm): 100 Fraction size:
1.00
ml
UV range (AU):
Tube number:
START
STOP
ON
Advance
Set START
2.0 Event mark
Volume left:
OFF
STOP
SV3-2 at port 1
1
2
Gradient Pump 0.00 ml/min
0 %B 1 psi Flowrate of the gradient pump
UV
Conductivity
0.00889 AU
3,57 mS/cm
SIM1/SIG
Fig. 6. Manual control screen for a Manual BioLogic HR System.
17
SIM2/pH
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4. Control of the BioLogic HR Pumps. The gradient pump parameters are set from the manual screen either by clicking in the appropriate field and entering a value from the keyboard or by using the spin arrows. You can alter the flow rate from 0.1 to 10 ml/min for any given proportion of pumps A and B. Note that the total flow rate can not exceed 10 ml/min (i.e. with a set flow-rate of 10 ml/min at 50% B, both pump heads A and B are delivering at 5 ml/min each). To start the pump, click the Start button. Note the running man icon. To change the pump parameters while the pump is running, enter the new value and then click on the Set button. The maximum pressure capability of the BioLogic HR gradient pumps is 1000 psi. Pressure limits can be adjusted to match the pressure limits of a column. If the pressure limit is exceeded, the pump will stop and an alarm will sound. For now, set the high limit to 700 psi and the low limit to 20 psi. 5. Flushing the System through to the fraction collector. With the gradient pumps stopped, move the inject valve back to position L (Load) by either moving the lever to the right (V7-3) or clicking radio button L (AV7-3) on the Manual Screen. Using the Manual Screen, set the pump flow rate at 1.0 ml/min and start the pump. Water will flow through the UV and conductivity flow cells and to the fraction collector, as described below. a. Using the Model 2110 Fraction Collector and SV3-2 valve as a diverter valve. If you plugged the SV3-2 valve into Solenoid valve port 1, you will see a valve box on the Manual Screen designated SV3-2 at port 1. (see Figure 2) The two radio buttons of this box correspond to valve positions; 1 = Waste, 2 = Collect. Select position 1 (waste) to divert the flow to waste. The fraction collector box on the manual screen (refer to Figure 2) will show fields for fraction size–ml, Tube number, Volume left, a toggle button for Start and Stop and a button for Advance. Note that tube number is a display field only. •
Place tubes in the fraction collector rack and set a fraction size of 1 ml. Click on the Start button and select valve position 2 of the SV3-2 valve box. Flow will now be diverted to the fraction collector tubes. Click the Advance button to test its function if desired. 18
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Continue to pump water through the system for at least 10 minutes. You may wish to continue fraction collection or return the SV3-2 valve to position 1 and then stop fraction collection.
Note: In manual operation, starting or stopping fraction collection does not change the SV3-2 diverter valve position. You must always manually set the SV3-2 valve to the waste or collect position. b. Using a Model 2128 Fraction Collector. The Model 2128 Fraction Collector has two operating modes: •
System: Controlled by the BioLogic HR System.
•
Local: Controlled from its own faceplate.
For now, insure that the System button is selected. When in System mode, operation of the fraction collector is as follows. •
Control of the Model 2128 is identical regardless of whether or not the optional on-arm diverter valve is used. Without a valve, the drop-head returns to the waste trough during divert operations.
•
The fraction collector box on the manual screen will show fields for Rack type, Start tube, End tube, Fraction size–ml, Tube number, Volume left, a toggle button for Start and Stop and a button for Advance (see Figure 7).
BioLogicHR - Default - no method File View Utilities Options New
Browser Report
Gradient pump
Inlet B: High limit: Low limit:
Help 1 2
Run
wash load
Manual Setup Protocol
Run
Notes PostRun
100
Log
ON
UV Detector
Fraction Collector
Zero Baseline
System Local ml/min Mode: Rack: Rack 1 (128 tubes)
Flow rate: 1.00 Inlet A:
Window
New
Edit
Method Method
ON
OFF
%
0
%
1000
psi
0
psi
Start Tube:
1
End Tube:
128
Fraction size:
1.00
Tube number:
1
Chart Recorder Conductivity range(mS/cm): 500 ml
UV range (AU):
Volume left:
ON
Advance
Set
0.1 Event mark OFF
Signal Import Module START
STOP
START
STOP SIM 1 and SIM 2 connected
SV3-2 at port 1
SV5-4 at port 2
AV7-3 at port 4
AV9-8 at port 5
I 1 1
2
L 4
I
2
3
P
8
2
6
4
7
3
5
Gradient Pump
UV
Conductivity
SIM1/SIG
SIM2/pH
0 %B 438 psi Flowrate of the gradient pump
-0.00181 AU
47.5 mS/cm
0.089 Volt
7.00 pH
0.00 ml/min
Fig. 7. Manual Control Screen for the Automated BioLogic System.
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