Applied Biosystems 7500/7500 Fast: Real-Time PCR Systems
Applied Biosystems 7500/7500 Fast: Real-Time PCR Systems
Applied Biosystems 7500/7500 Fast: Real-Time PCR Systems
Applied Biosystems
7500/7500 Fast
Real-Time PCR Systems
System Maintenance
Maintenance Guide
Overview
Applied Biosystems
7500/7500 Fast
Real-Time PCR Systems Perform the
Regions of Interest
(ROI) Calibration
System Maintenance
Perform the
Background
Calibration and
Optical Calibration
Verify the
Instrument
Performance
User-Performed
Maintenance
© Copyright 2008, 2010 Applied Biosystems. All rights reserved.
Information in this document is subject to change without notice. Applied Biosystems assumes no responsibility for any errors that may appear in this
document.
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THIS DOCUMENT, INCLUDING BUT NOT LIMITED TO THE USE THEREOF.
NOTICE TO PURCHASER: Label License
The Applied Biosystems 7500 and 7500 Fast Real-Time PCR Systems are covered by US patents and corresponding claims in their non-US counterparts,
owned by Applied Biosystems. No right is conveyed expressly, by implication, or by estoppel under any other patent claim, such as claims to apparatus, re-
agents, kits, or methods such as 5′ nuclease methods. Further information on purchasing licenses may be obtained by contacting the Director of Licensing,
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TRADEMARKS:
Applera, Applied Biosystems, AB (Design), ABI PRISM, and VIC are registered trademarks, and FAM, JOE, NED, ROX, and TAMRA are trademarks of
Applied Biosystems or its subsidiaries in the U.S. and/or certain other countries.
AmpErase and TaqMan are registered trademarks of Roche Molecular Systems, Inc.
SYBR is a registered trademark of Molecular Probes, Inc.
Microsoft and Windows are registered trademarks of Microsoft Corporation.
All other trademarks are the sole property of their respective owners.
Preface . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . vii
How to Use This Guide . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . vii
How to Obtain More Information . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . viii
How to Obtain Support . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . x
Chapter 1 Overview . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 1
About the 7500/7500 Fast System . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 2
How to Use This Guide . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 4
Recommended Maintenance Schedule . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 5
Maintain the Computer Hard Drive(s) . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 6
Archive and Back Up EDS Files . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 6
Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide iii
Chapter 3 Perform the Background Calibration and Optical
Calibration . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 19
Perform the Background Calibration . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 20
Prepare the Background Calibration Plate . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 21
Perform the Background Calibration . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 23
Perform the Optical Calibration . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 25
Prepare the Calibration Plate . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 25
Perform the Optical Calibration . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 28
Troubleshoot the Background Calibration . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 30
Index . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 83
Audience This guide is intended for novice and experienced 7500/7500 Fast system users who
need to maintain their system.
Assumptions This guide assumes that your 7500/7500 Fast system has been installed by an
Applied Biosystems technical representative and that you:
• Are familiar with the Microsoft® Windows® operating system.
• Understand general techniques for preparing and handling DNA samples.
• Have a general understanding of hard drives and data storage, file transfers, and
copying and pasting.
User Attention Two user attention words appear in Applied Biosystems user documentation. Each word
Words implies a particular level of observation or action as described below:
Note: – Provides information that may be of interest or help but is not critical to the use
of the product.
Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide vii
Preface
How to Obtain More Information
IMPORTANT! To verify your client connection to the database, you need a valid user ID
and password.
Safety Alert Safety alert words also appear in user documentation. For more information, see “Safety
Words Alert Words” on page xii.
Applied Biosystems 7500/7500 Fast Explains how to perform experiments on the 7500/7500 Fast 4387784
Real-Time PCR System Getting Started system. Each Getting Started Guide functions as both:
Guide for Genotyping Experiments
• Tutorial, using example experiment data provided with the
Applied Biosystems 7500/7500 Fast Applied Biosystems 7500/7500 Fast Real-Time PCR 4387785
Real-Time PCR System Getting Started Software (7500 Software).
Guide for Presence/Absence Experiments • Guide for your own experiments.
Intended for laboratory staff and principal investigators who
Applied Biosystems 7500/7500 Fast 4387783
perform experiments using the 7500/7500 Fast system.
Real-Time PCR System Getting Started
Guide for Relative Standard Curve and
Comparative CT Experiments
Applied Biosystems 7500/7500 Fast Explains how to install and maintain the 7500/7500 Fast system. 4387777
Real-Time PCR System Maintenance
Intended for laboratory staff responsible for the installation and
Guide
maintenance of the 7500/7500 Fast system.
Applied Biosystems 7500/7500 Fast 4387778
Real-Time PCR System Computer Setup
Guide
Applied Biosystems 7500/7500 Fast Provides information about the reagents you can use on the 4387787
Real-Time PCR System Reagent Guide 7500/7500 Fast system, including:
• An introduction to TaqMan® and SYBR® Green reagents
• Descriptions and design guidelines for the following
experiment types:
– Quantitation experiments
– Genotyping experiments
– Presence/absence experiments
Intended for laboratory staff and principal investigators who
perform experiments using the 7500/7500 Fast system.
viii Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide
Preface
How to Obtain More Information
Applied Biosystems 7500/7500 Fast Explains how to prepare your site to receive and install the 4387776
Real-Time PCR System Site Preparation 7500/7500 Fast system.
Guide
Intended for personnel who schedule, manage, and perform the
tasks required to prepare your site for installation of the
7500/7500 Fast system.
Applied Biosystems 7500/7500 Fast Explains how to use the 7500 Software to: NA
Real-Time PCR Software v2.0 Help
• Set up, run, and analyze experiments using the 7500/7500
Fast system.
• Monitor a networked 7500/7500 Fast instrument.
• Calibrate a 7500/7500 Fast instrument.
• Verify the performance of a 7500/7500 Fast instrument with
an RNase P run.
Intended for:
• Laboratory staff and principal investigators who perform
experiments using the 7500/7500 Fast system.
• Laboratory staff responsible for the installation and
maintenance of the 7500/7500 Fast system.
Note: To open the user documentation included on the Documentation CD, use the
Adobe® Acrobat® Reader® software available from www.adobe.com.
Obtaining The 7500 software has a Help system that describes how to use each feature of the user
Information from interface. Access the Help system by doing one of the following:
the Help System • Click in the toolbar of the 7500 software window
• Select Help 7500 Software Help
• Press F1
You can use the Help system to find topics of interest by:
• Reviewing the table of contents
• Searching for a specific topic
• Searching an alphabetized index
You can also access PDF versions of all documents in the Applied Biosystems
7500/7500 Fast Real-Time PCR System document set from the Help system.
Send Us Your Applied Biosystems welcomes your comments and suggestions for improving its user
Comments documents. You can e-mail your comments to:
[email protected]
IMPORTANT! The e-mail address above is only for submitting comments and
suggestions relating to documentation. To order documents, download PDF files, or for
help with a technical question, go to www.appliedbiosystems.com, then click the link
for Support. (See “How to Obtain Support” below).
Definitions
Examples
The following examples show the use of safety alert words:
IMPORTANT! Wear powder-free gloves when you handle the halogen lamp.
The lamp is extremely hot. Do not touch the lamp until it has cooled to
room temperature.
xii Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide
Safety and EMC Compliance Information
Symbols on Instruments
Symbols on Instruments
Electrical The following table describes the electrical symbols that may be displayed on
Symbols on Applied Biosystems instruments.
Instruments
Symbol Description Symbol Description
Safety Symbols The following table describes the safety symbols that may be displayed on
Applied Biosystems instruments. Each symbol may appear by itself or in combination
with text that explains the relevant hazard (see “Safety Labels on Instruments” on
page xiv). These safety symbols may also appear next to DANGERS, WARNINGS, and
CAUTIONS that occur in the text of this and other product-support documents.
Symbol Description
Indicates that you should consult the manual for further information and to
proceed with appropriate caution.
Indicates the presence of a laser inside the instrument and to proceed with
appropriate caution.
Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide xiii
Safety and EMC Compliance Information
Safety Labels on Instruments
Environmental The following symbol applies to all Applied Biosystems electrical and electronic
Symbols on products placed on the European market after August 13, 2005.
Instruments
Symbol Description
English Français
WARNING To reduce the chance of electrical AVERTISSEMENT Pour éviter les risques
shock, do not remove covers that require tool d'électrocution, ne pas retirer les capots dont
access. No user-serviceable parts are inside. l'ouverture nécessite l'utilisation d'outils.
Refer servicing to Applied Biosystems L’instrument ne contient aucune pièce
qualified service personnel. réparable par l’utilisateur. Toute intervention
doit être effectuée par le personnel de service
qualifié de Applied Biosystems.
WARNING This instrument is designed for AVERTISSEMENT Cet instrument est conçu
12V, 75W Halogen lamps only. pour des lampes d'halogène de 12V et 75W
seulement.
xiv Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide
Safety and EMC Compliance Information
Safety Labels on Instruments
Locations of The Applied Biosystems 7500/7500 Fast Real-Time PCR System contains warnings at
Warnings the locations shown below.
Attention
Physical hazard
Physical hazard
Attention
Attention
Attention
Moving and Do not attempt to lift or move the computer or the monitor without
Lifting the assistance of others. Depending on the weight of the computer and/or the monitor,
Stand-Alone moving them may require two or more people.
Computers and
Monitors Things to consider before lifting the computer and/or the monitor:
• Make sure that you have a secure, comfortable grip on the computer or the monitor
when lifting.
• Make sure that the path from where the object is to where it is being moved is clear
of obstructions.
• Do not lift an object and twist your torso at the same time.
• Keep your spine in a good neutral position while lifting with your legs.
• Participants should coordinate lift and move intentions with each other before
lifting and carrying.
• Instead of lifting the object from the packing box, carefully tilt the box on its side
and hold it stationary while someone slides the contents out of the box.
Operating the Ensure that anyone who operates the instrument has:
Instrument • Received instructions in both general safety practices for laboratories and specific
safety practices for the instrument.
• Read and understood all applicable Material Safety Data Sheets (MSDSs). See
“About MSDSs” on page xvii.
xvi Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide
Safety and EMC Compliance Information
Chemical Safety
Chemical Safety
Chemical Hazard CHEMICAL HAZARD. Before handling any chemicals, refer to
Warning the Material Safety Data Sheet (MSDS) provided by the manufacturer, and observe all
relevant precautions.
About MSDSs Chemical manufacturers supply current Material Safety Data Sheets (MSDSs) with
shipments of hazardous chemicals to new customers. They also provide MSDSs with the
first shipment of a hazardous chemical to a customer after an MSDS has been updated.
MSDSs provide the safety information you need to store, handle, transport, and dispose
of the chemicals safely.
Each time you receive a new MSDS packaged with a hazardous chemical, be sure to
replace the appropriate MSDS in your files.
Obtaining MSDSs The MSDS for any chemical supplied by Applied Biosystems is available to you free
24 hours a day. To obtain MSDSs:
1. Go to www.appliedbiosystems.com, click Support, then click MSDS Search.
2. In the Keyword Search field, enter the chemical name, product name, MSDS part
number, or other information that appears in the MSDS of interest. Select the
language of your choice, then click Search.
3. Find the document of interest, right-click the document title, then select any of the
following:
• Open – To view the document
• Print Target – To print the document
• Save Target As – To download a PDF version of the document to a destination
that you choose
Note: For the MSDSs of chemicals not distributed by Applied Biosystems, contact the
chemical manufacturer.
Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide xvii
Safety and EMC Compliance Information
Chemical Safety
xviii Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide
Safety and EMC Compliance Information
Chemical Waste Safety
Waste Disposal If potentially hazardous waste is generated when you operate the instrument, you must:
• Characterize (by analysis if necessary) the waste generated by the particular
applications, reagents, and substrates used in your laboratory.
• Ensure the health and safety of all personnel in your laboratory.
• Ensure that the instrument waste is stored, transferred, transported, and disposed of
according to all local, state/provincial, and/or national regulations.
Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide xix
Safety and EMC Compliance Information
Electrical Safety
Electrical Safety
Overvoltage The Applied Biosystems 7500/7500 Fast Real-Time PCR System has an installation
Rating (overvoltage) category of II, and is classified as portable equipment.
Workstation Safety
Correct ergonomic configuration of your workstation can reduce or prevent effects such
as fatigue, pain, and strain. Minimize or eliminate these effects by configuring your
workstation to promote neutral or relaxed working positions.
Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide xxi
Safety and EMC Compliance Information
Safety and Electromagnetic Compatibility (EMC) Standards
U.S. and This instrument has been tested to and complies with standard UL 61010A-1, “Safety
Canadian Safety Requirements for Electrical Equipment for Laboratory Use, Part 1: General
Standards Requirements” and with standard UL 61010-2-010, “Particular Requirements for
Laboratory Equipment for the Heating of Materials.”
This instrument has been tested to and complies with standard CSA 1010.1, “Safety
Requirements for Electrical Equipment for Measurement, Control, and Laboratory Use,
Part 1: General Requirements.”
Canadian EMC This instrument has been tested to and complies with ICES-001, Issue 3: Industrial,
Standard Scientific, and Medical Radio Frequency Generators.
EMC
This instrument meets European requirements for emission and immunity (EMC
Directive 2004/108/EC). This instrument has been tested to and complies with standard
EN 61326 (Group 1, Class B), “Electrical Equipment for Measurement, Control and
Laboratory Use – EMC Requirements.”
Australian EMC This instrument has been tested to and complies with standard AS/NZS 2064, “Limits
Standards and Methods Measurement of Electromagnetic Disturbance Characteristics of Industrial,
Scientific, and Medical (ISM) Radio-frequency Equipment.”
xxii Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide
Chapter 1
X-
Overview
Note: For more information about any of the topics discussed in this guide, access the
Help from within Applied Biosystems 7500/7500 Fast Real-Time PCR System Software
v2.0 by pressing F1, clicking in the toolbar, or selecting Help 7500 Software Help.
Notes
About Data The 7500/7500 Fast system collects raw fluorescence data at different points during a
Collection PCR, depending on the type of run that the instrument performs:
Real-time Standard curve The instrument collects data following each extension
runs step of the PCR.
Relative standard
curve
Comparative CT
(ΔΔCT)
Regardless of the run type, a data collection point or read on the 7500/7500 Fast
instrument consists of three phases:
1. Excitation – The instrument illuminates all wells of the reaction plate, exciting the
fluorophores in each reaction.
2. Emission – The instrument optics collect the residual fluorescence emitted from the
wells of the reaction plate. The resulting image consists only of light that
corresponds to the range of emission wavelengths.
Notes
About the Filters The 7500/7500 Fast system uses five filters to support the following system dyes:
• FAM™ dye • JOE™ dye • TAMRA™ dye • ROX™ dye Cy5® dye
• SYBR® • VIC® dye • NED™ dye • Texas Red®
Green dye • CY3® dye dye
Note: To access the Help, select Help 7500 Software Help from within the 7500
software.
Notes
Chapter/
Title Description
Appendix
A Store, Move, and Install Describes how to store, move, and reinstall the
the 7500/7500 Fast components of the 7500/7500 Fast system.
System
B Create a Custom Dye Describes how to create a dye plate that can be used
Plate to calibrate the 7500/7500 Fast system for a dye not
manufactured by Applied Biosystems.
Notes
IMPORTANT! The numbered lists in the table below indicate that the tasks must be
performed in sequence.
Monthly 1. Check the lamp status. If necessary, replace the halogen lamp. 58
2. Perform a background calibration. ‡
20
3. Run disk cleanup and disk defragmentation. 6
Semiannually 1. Check the lamp status. If necessary, replace the halogen lamp. 58
(6 Months)
2. Perform a regions of interest (ROI) calibration. 7
3. Perform a background calibration. 20
4. Perform an optical calibration. 25
5. Perform a dye calibration. 31
6. Perform an RNase P instrument verification run. 45
‡ You can perform a background calibration to check for contamination. If any parts of the optics are
replaced or moved, you must run an ROI calibration, a background calibration, an optical calibration,
a dye calibration, and an RNase P instrument verification run.
Notes
For More In the desktop, select Start Help and Support to access the Help for the Windows
Information operating system. Use the search function of the Help to find information on the
“Disk Cleanup” and “Disk Defragment” utilities.
IMPORTANT! Do not run the disk management utilities and 7500 software at the same
time.
Back Up EDS Applied Biosystems strongly recommends that you back up your experiments.
Files
Backing up data:
• Protects against potential loss of data caused by an unforeseen failure of the
computer or its hard drive(s).
• Conserves space on the hard drive and optimizes performance, if you remove old
data after backing up.
Develop a Data Applied Biosystems recommends developing a strategy for managing the files produced
Management by the 7500 software.
Strategy
Note: Real-time runs generate significantly more data than genotyping or
presence/absence experiments. During one day of real-time operation, the 7500/7500
Fast system can generate more than 10 MB of data.
Check Disk If you perform real-time experiments on your 7500/7500 Fast system, check the amount
Space of available space on your hard drive weekly. When the hard drive is within 20% of
maximum capacity, transfer the older data to a backup storage device.
Notes
Note: For more information about any of the topics discussed in this guide, access the
Help from within Applied Biosystems 7500/7500 Fast Real-Time PCR System Software
v2.0 by pressing F1, clicking in the toolbar, or selecting Help 7500 Software Help.
Notes
Overview
A regions of interest (ROI) calibration maps the positions of the wells on the sample
block of the Applied Biosystems 7500/7500 Fast Real-Time PCR System. The 7500
software uses the ROI calibration data to associate increases in fluorescence during a run
with specific wells of the plate. The instrument uses a set of optic filters to distinguish
the fluorescence emissions gathered during runs. You must generate a calibration image
for each individual filter to account for minor differences in the optical path.
Materials
Required
Safety GR2170
IMPORTANT! After every ROI calibration, you must perform a background calibration,
optical calibration, dye calibration, and instrument verification.
Notes
A1 at
notched
A1 at corner
top-left
opposite
corner
from
notched
top-right
corner (A12).
30-µL
100-µL maximum
maximum reaction
reaction volume
Vortex standard plates to ensure complete Centrifuge Fast plates to ensure that all
mixing, then centrifuge to ensure that all reagents are in the bottom of the well.
reagents are contained in the bottom of the Do not vortex Fast plates. Vortexing can
well. cause loss of smaller reaction volumes.
Prepare the Plate IMPORTANT! Wear powder-free gloves when you handle the ROI calibration plate.
1. Obtain the ROI calibration plate from the spectral calibration kit in the freezer.
2. Allow the ROI calibration plate to warm to room temperature (approximately 5 min).
IMPORTANT! Do not remove an ROI calibration plate from its packaging until you
are ready to run it. The fluorescent dye in the wells of the plate is photosensitive.
Prolonged exposure to light can diminish the fluorescence from the plate.
Notes
3. Remove the ROI calibration plate from its packaging. Leave the optical film on the
plate.
IMPORTANT! Do not discard the packaging for the ROI calibration plate. The plate
can be used up to three times if it is stored in its original packaging sleeve.
4. (Standard plates only) Vortex the ROI calibration plate for 5 sec.
IMPORTANT! The ROI calibration plate must be well mixed and centrifuged.
6. Verify that the liquid in each well of the ROI calibration plate is at the bottom of the
well. If not, centrifuge the plate again at a higher rpm and for a longer period of time.
Correct Incorrect
Notes
Load the Plate PHYSICAL INJURY HAZARD. During instrument operation, the
sample block can be heated to 100 °C. Before performing the following procedure, be
sure to wait until the sample block reaches room temperature.
2. Load the plate into the plate holder in the instrument. Ensure that the plate is
properly aligned in the holder.
GR2475
5742RG
1 2 3 4 5 6 7 8 9 10 11 12
21 11 01 9 8 7 6 5 4 3 2 1
A
A
B
B
C
C
D
D
E
E
F
F
G
G
H
H
1 1
A A
GR2475
5742RG
7500
GR2477
0057
keyed corner
renroc deyek
3. Close the tray door. Apply pressure to the right side of the tray door at an angle.
GR2471
GR2471
7500
tray top view
Push
Notes
Start the 1. In the 7500 software, select Instrument Instrument Maintenance Manager.
Calibration
2. In the ROI screen of the Instrument Maintenance Manager, click Start Calibration.
Notes
Start the 1. In the 7500 software, select Instrument Instrument Maintenance Manager.
Calibration
2. In the ROI tab of the Instrument Maintenance Manager, click Start Manual
Calibration.
3a
3b
5. Determine if your ROI image is acceptable (the figures below show unsaturated and
oversaturated images). Wells in an acceptable image:
• Must be as bright as possible without oversaturating. (When you generate the
ROI calibration, a warning is displayed if wells are oversaturated.)
• Can contain some, but do not have to contain any, red pixels, which represent
saturation.
Normal Over
Unsaturated
Saturation Saturated
Notes
a. Click OK.
b. Decrease the Exposure Time by
half (see step 3a on page 13).
c. Repeat steps 3 and 5.
or
A very faint ROI image, or you cannot generate a See “Troubleshoot the ROI Calibration”
successful calibration. on page 17.
Successful
calibration –
Wells Found
must be 96
• ROI Image displays a green circle
around each well area.
Notes
9. Repeat steps 3 through 8 for the remaining filters, resetting the Exposure Time to
2048 before performing the calibration for each filter. The ROI calibration is
complete when Filter Masks Loaded for all the filters displays OK.
Notes
Unload the Plate PHYSICAL INJURY HAZARD. During instrument operation, the
sample block can be heated to 100 °C. Before performing the following procedure, be
sure to wait until the sample block reaches room temperature.
GR2471
GR2477
7300/7500
barcode on plate
GR2471
7500
tray top view
Push
GR2477
2. Place the calibration plate inside its packaging sleeve. If you plan to perform
background and optical calibrations:
• Within the next 8 hr, keep the ROI calibration plate at room temperature. The
optical calibration uses the ROI calibration plate.
• On another day, return the packaged plate to the spectral calibration kit in the
freezer.
IMPORTANT! Do not discard the calibration plate. If the plate is stored in its
original packaging sleeve, you can use it up to three times after you open it.
IMPORTANT! After you perform an ROI calibration, you must also perform a
background calibration (see page 20), an optical calibration (see page 25), dye
calibrations (see page 32), and instrument verification (see page 46).
Notes
ROI Calibration The sample block may be 1. If the CCD Control Settings in the ROI Inspector displays
Failed in its lowered position. “Block Up,” click Block Up, to raise the block.
Click
2. Check that the heated cover assembly is pulled all the way forward
to ensure that the tray can be pushed in properly. If the 7500/7500
ROI Image is Faint Fast system has a heated cover latch installed, check that the latch
is in a locked position.
Heated cover
assembly
GR2482 GR2482
7500/7500 fast
heated cover assembly
Notes
Notes
Note: For more information about any of the topics discussed in this guide, access the
Help from within Applied Biosystems 7500/7500 Fast Real-Time PCR System Software
v2.0 by pressing F1, clicking in the toolbar, or selecting Help 7500 Software Help.
Notes
Materials Background
Required Plate Safety
goggles
GR2170
Background Fluorescence data collected by the 7500/7500 Fast system includes a fluorescence signal
Fluorescence inherent to the system, referred to as background fluorescence. Background fluorescence
is a composite signal found in all spectral data. This signal consists of fluorescence from
several sources, including:
• Background electronic signal
• Contaminants in the sample block
• The plastic consumable (plates and caps)
Guidelines for • Make sure the centrifuge you use is clean. Before centrifuging, wipe down the
Calibration bucket using a tissue.
• Handle the calibration plates with care to prevent contamination. Do not place plates
on a lab bench, which may contaminate the plate. Always put calibration plates back
into their original bags.
Notes
Prepare the Plate IMPORTANT! Wear powder-free gloves when you handle the plate.
1. Obtain the prepared background plate from the spectral calibration kit in the freezer.
2. Allow the background plate to warm to room temperature (at least 5 min).
IMPORTANT! Do not discard the packaging for the plate. The background plate can
be used up to three times if it is stored in its original packaging sleeve.
6. Verify that the liquid in each well of the background plate is at the bottom of the well.
If not, centrifuge the plate again at a higher rpm and for a longer period of time.
IMPORTANT! Do not allow the bottom of the background plate to become dirty.
Fluids and other contaminants that adhere to the bottom of the plate can contaminate
the sample block and cause an abnormally high background signal.
Correct Incorrect
Notes
Load the Plate PHYSICAL INJURY HAZARD. During instrument operation, the
sample block can be heated to 100 °C. Before performing the following procedure, be
sure to wait until the sample block reaches room temperature.
2. Load the plate into the plate holder in the instrument. Ensure that the plate is
properly aligned in the holder.
GR2475
5742RG
1 2 3 4 5 6 7 8 9 10 11 12
21 11 01 9 8 7 6 5 4 3 2 1
A
A
B
B
C
C
D
D
E
E
F
F
G
G
H
H
1 1
A A
GR2475
5742RG
7500
GR2477
0057
keyed corner
renroc deyek
3. Close the tray door. Apply pressure to the right side of the tray door at an angle.
GR2471
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tray top view
Push
Note: If you cannot open the tray, the sample block may be in its raised position, locking the
tray door position. To lower the block, select Instrument Calibrate, then exit the ROI
Inspector.
Notes
Perform the 1. In the 7500 software, select Instrument Instrument Maintenance Manager.
Calibration
2. In the Instrument Maintenance Manager, select the Background tab.
Note: Before starting the calibration, the instrument may pause (up to 10 min) to allow
the heated cover to reach temperature.
Notes
Unload the Plate PHYSICAL INJURY HAZARD. During instrument operation, the
sample block can be heated to 100 °C. Before performing the following procedure, be
sure to wait until the sample block reaches room temperature.
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2. Place the calibration plate inside its packaging sleeve, then return the packaged plate
to the spectral calibration kit in the freezer.
IMPORTANT! Do not discard the calibration plate. If the plate is stored in its
original packaging sleeve, you can use the plate up to three times after you open it.
Notes
Prepare the Plate If you kept your ROI calibration plate at room temperature after performing an ROI
calibration (see Chapter 2), skip to step 5 on page 26 to spin down any condensation that may
have formed when the plate was at room temperature. If the ROI calibration plate is in the
freezer, go to step 1.
1. Obtain the ROI calibration plate from the spectral calibration kit in the freezer.
2. Allow the ROI calibration plate to warm to room temperature (at least 5 min).
IMPORTANT! Do not discard the packaging for the plate. The ROI calibration plate
can be used up to three times if it is stored in its original packaging sleeve.
Notes
IMPORTANT! The ROI calibration plate must be well mixed and centrifuged.
6. Verify that the liquid in each well of the ROI calibration plate is at the bottom of the
well. If not, centrifuge the plate again at a higher rpm and for a longer period of time.
Correct Incorrect
Notes
Load the Plate PHYSICAL INJURY HAZARD. During instrument operation, the
sample block can be heated to 100 °C. Before performing the following procedure, be
sure to wait until the sample block reaches room temperature.
2. Load the plate into the plate holder in the instrument. Ensure that the plate is
properly aligned in the holder.
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3. Close the tray door. Apply pressure to the right side of the tray door at an angle.
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Notes
Perform the 1. In the 7500 software, select Instrument Instrument Maintenance Manager.
Calibration
2. In the Instrument Maintenance Manager, select the Optical tab.
Note: Before starting the calibration, the instrument may pause (up to 10 min) to allow
the heated cover to reach temperature.
Unload the Plate PHYSICAL INJURY HAZARD. During instrument operation, the
sample block can be heated to 100 °C. Before performing the following procedure, be
sure to wait until the sample block reaches room temperature.
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Notes
2. Place the calibration plate inside its packaging sleeve. Return the packaged plate to
the spectral calibration kit in the freezer.
IMPORTANT! Do not discard the calibration plate. If the plate is stored in its
original packaging sleeve, you can use it up to three times after you open it.
Notes
Background One or more wells of the 1. Repeat the calibration using the same background plate.
Calibration Failed background plate produced
2. If the calibration fails again, repeat the calibration using a
spectra that exceed the
different background plate.
maximum limit for the
instrument. 3. If the calibration fails again, determine the source of the
contamination, as explained in “How to Identify
Contamination” below.
How to Identify Signals that exceed the limit of normal background fluorescence may indicate
Contamination fluorescent contaminants on the calibration plate or the sample block. Common
contaminants include ink residue from permanent pens, powder from disposable gloves,
and dust.
1. While viewing the raw spectra, locate the contaminated well position(s) by selecting
successively smaller regions of the plate layout.
2. Rotate the background plate 180°, then perform the background calibration again.
1. Load a plate covered by a piece of black paper into the 7500/7500 Fast instrument.
3. After the run is complete, select all wells of the plate layout.
Notes
Note: For more information about any of the topics discussed in this guide, access the
Help from within Applied Biosystems 7500/7500 Fast Real-Time PCR System Software
v2.0 by pressing F1, clicking in the toolbar, or selecting Help 7500 Software Help.
Notes
Overview
During a dye calibration, the Applied Biosystems 7500/7500 Fast Real-Time PCR System:
• Collects spectral data from a series of dye standards.
• Stores the spectral information for the dye standards in a pure spectra calibration file.
The software uses the pure spectra data during experiment runs to characterize and
distinguish the individual contribution of each dye in the total fluorescence collected by
the instrument. After each run, the 7500 software receives data in the form of a raw
spectra signal for each reading. It determines the contribution of each fluorescent dye
used in the sample by comparing the raw spectra to the pure spectra calibration data.
When you save an experiment after analysis, the software stores the pure spectra with the
collected fluorescence data for that experiment.
Time Required 1 hr
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Dye Plates
Powder-free Centrifuge with
(CY3 , CY5 , FAM , JOE™, NED™, ROX™, SYBR®
® ® ™
gloves plate adapter
Green, TAMRA™, TEXAS RED®, and VIC® dyes)
Note: If you store Applied Biosystems 7500/7500 Fast Real-Time PCR System dye
plates in their original packaging in the freezer, you can use them to calibrate a
7500/7500 Fast instrument up to 3 times for 6 months after opening them.
IMPORTANT! You must perform a background run before every series of dye
calibrations. Because the age and use of instrument components can affect pure spectra
readings, Applied Biosystems recommends performing a dye calibration at least every
6 months.
Notes
Dye Sets The Applied Biosystems 7500/7500 Fast Real-Time PCR Systems use the following dye
sets for calibration: CY3® dye, CY5® dye, FAM™ dye, JOE™ dye, NED™ dye, ROX™ dye,
SYBR® Green dye, TAMRA™ dye, TEXAS RED® dye, and VIC® dye. The following
figure shows the emission spectrum for each dye, and the filters and wavelengths at
which each dye is read.
Filters 1 2 3 4 5
Spectrum
500 600 700
(nm)
Emission
Spectra
Custom Dye The 7500/7500 Fast system can be used to run assays designed with custom dyes (dyes
not supplied by Applied Biosystems). However, before using custom dyes with the
7500/7500 Fast instrument, you must create and run a custom calibration plate. The 7500
software uses the custom calibration plate to create a spectral standard to distinguish the
custom dye in the fluorescence data collected during the run. See Appendix B for
information on custom dye calibrations.
IMPORTANT! To use a custom dye on your 7500/7500 Fast system, it must fluoresce
within the 520 to 650 nm spectral range measured by the 7500/7500 Fast instrument.
Notes
About the The product of a dye calibration is a collection of spectral profiles that represent the
Analysis fluorescence signature of each dye standard. Each profile consists of a set of spectra that
correspond to the fluorescence collected from the wells of the spectral calibration plate.
The 7500 software plots the resulting data for each spectral profile in a graph of
fluorescence versus filter.
When the 7500 software extracts the calibration data from a dye run, it evaluates the
fluorescence signal generated by each well in terms of the collective spectra for the entire
calibration plate. Dye spectra are generally acceptable if they peak within the same filter
as their group but diverge slightly at other wavelengths (see below).
The 7500 software can compensate for some differences in a spectral profile by replacing
(auto-repairing) the spectra of unacceptable wells with the spectra of other wells on the
reaction plate. However, the software allows only a few replacements and may reject the
calibration if the spectra between neighboring wells vary significantly.
Note: Because the wells in a calibration plate contain dyes at identical concentrations,
the resulting signals for the wells containing each dye should be similar. Among wells
containing the same dye, variations in spectral position and peak position are caused by
minor differences in the optical properties and excitation energy between the individual
wells.
Acceptable Spectra
Spectra peak at the same wavelength and
do not diverge significantly
Unacceptable Spectra
Spectra peak at the different wavelengths
Notes
Prepare the IMPORTANT! Wear powder-free gloves when you handle the plate.
Plates
1. Obtain the spectral calibration kit from the freezer, then remove all of the dye plates.
IMPORTANT! Do not remove a dye plate from its packaging until you are ready to run it.
The fluorescent dye in the wells of each dye plate is photosensitive. Prolonged exposure
to light can diminish the fluorescence signal strength of the plate.
Note: If you store Applied Biosystems 7500/7500 Fast Real-Time PCR System dye
plates in their original packaging in the freezer, you can use them to calibrate a
7500/7500 Fast instrument up to 3 times for 6 months after opening them.
Notes
IMPORTANT! The wizard guides you through the calibration of each dye separately.
You must set up, run, and analyze each dye plate independently.
Note: Before starting the calibration, the instrument may pause (up to 10 min) to
allow the heated cover to reach temperature.
Notes
Load a Dye Plate Note: Because the wizard guides you through the calibration of each dye separately,
perform the following procedure for each dye that you calibrate.
1. Remove the dye plate that is specified by the software from its packaging.
IMPORTANT! Do not discard the packaging for the plate. The plate can be used up
to three times if it is stored in its original packaging sleeve.
4. Verify that the liquid in each well of the plate is at the bottom of the well. If not,
centrifuge the plate again at a higher rpm and for a longer period of time.
Correct Incorrect
5. Verify that the dye plate that you are about to load matches the dye selected in the
7500 software.
Dye label
Notes
7. Load the plate into the plate holder in the instrument. Ensure that the plate is
properly aligned in the holder.
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8. Close the tray door. Apply pressure to the right side of the tray door at an angle.
Note: If you cannot open the tray, the sample block may be in its raised position, locking the
tray position. To lower the block, select Instrument Calibrate, then exit the ROI Inspector.
Notes
Analyze the Note: Because the wizard guides you through the calibration of each dye separately,
Calibration Data perform the following procedure for each dye that you calibrate.
b. Inspect the raw data. For each spectrum, verify that the peak is:
• Within the detectable range for the 7500/7500 Fast instrument.
• Free of irregular spectral peaks.
• Present in the correct channel for the dye (see Table 1 on page 41).
If a spectrum does not match the criteria above, troubleshoot the problem as
described in “Troubleshoot the Dye Calibration” on page 43.
Note: Among wells containing the same dye, variations in spectral position and
peak position are caused by minor differences in the optical properties and
excitation energy between the individual wells.
2a
2b
Notes
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d. Place the calibration plate inside its packaging sleeve. Return the packaged
plate to the spectral calibration kit in the freezer.
Note: If you store Applied Biosystems 7500/7500 Fast Real-Time PCR System
dye plates in their original packaging in the freezer, you can use them to calibrate
7500/7500 Fast instruments up to 3 times for 6 months after opening them.
6. Prepare and run the next plate as explained in “Prepare the Plates” on page 35.
Notes
NED dye
VIC dye
7500/7500 Fast system dye spectra
FAM dye
CY3 dye
JOE dye
Peak (nm)
~520
~550
~580
Table 1
Filter
3
Notes
Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide 41
Chapter 4 Perform the Dye Calibration
Perform the Dye Calibration
TEXAS RED dye
Dye/Spectra
7500/7500 Fast system dye spectra
ROX dye
CY5 dye
Peak (nm)
~610
~670
Table 1
Filter
5
Notes
42 Applied Biosystems 7500/7500 Fast Real-Time PCR System Maintenance Guide
Chapter 4 Perform the Dye Calibration
Troubleshoot the Dye Calibration
One or more raw • The spectral calibration plate 1. Unload the 7500/7500 Fast instrument and view the wells of
spectra are at or was centrifuged insufficiently. the spectral calibration plate. If the liquid in the wells is not:
below the detectable • The spectral calibration plate – At the bottom of the wells, centrifuge the plate for a longer
threshold for the contains old or insufficient time, then repeat the calibration.
calibration. reagents. – Equivalent in volume, the plate is not sealed and the
• If you are running a custom reagents have evaporated. Discard it and run another.
spectral calibration plate, the
2. If the spectral calibration plate appears to be normal, discard
dye may not be present at a
the plate and run another.
sufficient concentration.
3. If the problem persists, contact Applied Biosystems as
explained in “How to Obtain Support” on page x.
Note: If you are running a custom spectral calibration plate,
create another plate but increase the concentration of the dye
that produced insufficient signal.
One or more raw • Fluorescent contaminants are Verify that contaminants are not present by performing a
spectra exceed the on the sample block(s) or background calibration as explained in Chapter 3, “Perform
maximum limit for the spectral calibration plate. the Background Calibration and Optical Calibration.” If the
7500/7500 Fast • If you are running a custom background calibration does not show sample block
instrument. spectral calibration plate, the contamination, the spectral calibration plate may be
dye may be too concentrated. contaminated.
Note: If you are running a custom spectral calibration plate,
The spectra contain Fluorescent contaminants are on create another plate but decrease the concentration of the dye
peaks in more than the sample block(s) or spectral that exceeds the detectable limit.
one filter. calibration plate.
Notes
Notes
Note: For more information about any of the topics discussed in this guide, access the
Help from within Applied Biosystems 7500/7500 Fast Real-Time PCR System Software
v2.0 by pressing F1, clicking in the toolbar, or selecting Help 7500 Software Help.
Notes
Overview
Perform the TaqMan® RNase P Instrument Verification Plate run to verify the
performance of an Applied Biosystems 7500/7500 Fast Real-Time PCR System.
Time Required 1 hr
GR2170
About the The RNase P plate is preloaded with the reagents necessary for the detection and quantitation
RNase P Plate of genomic copies of the human RNase P gene (a single-copy gene encoding the RNase
moiety of the RNase P enzyme).
Each well contains:
• 1✕ TaqMan® Fast Universal PCR Master Mix, No AmpErase® UNG
• RNase P primers
• FAM™ dye-labeled probe
• Known concentration of human genomic DNA template
The figure below illustrates the arrangement of the standard and unknown populations on
the RNase P plate. The RNase P plate contains five replicate groups of standards (1250,
2500, 5000, 10,000, and 20,000 copies), two unknown populations (5000 and 10,000
copies), and negative control wells (NC).
5K-copy Unknown
Population 1
10K-copy Unknown
Population 2
Notes
1. Generates a standard curve from the averaged threshold cycle (CT) values of the
replicate groups of standards.
2. Calculates the concentration of the two unknown populations using the standard
curve.
Installation Specification
The 7500/7500 Fast instrument passes the installation specification if the inequality
holds and the instrument successfully distinguishes between 5,000 and 10,000 copies
with a statistical confidence level of 99.7%.
To meet the installation specification, you can omit a limited number of outlier wells
from the 5,000- and 10,000-copy unknown populations.
7500 System
6 6 0 0
7500 Fast System
Notes
Prepare the IMPORTANT! Wear powder-free gloves when you handle the RNase P plate.
RNase P Plate
1. Obtain the TaqMan® RNase P Fast Instrument Verification Plate from the freezer, then
allow the reaction plate to warm to room temperature (for approximately 5 min).
5. Verify that the liquid is at the bottom of each well of the reaction plate. If not,
centrifuge the reaction plate again at a greater rpm and for a longer time.
IMPORTANT! Do not allow the bottom of the RNase P plate to become dirty. Fluids
and other contaminants that adhere to the bottom of the reaction plate can
contaminate the sample block(s) and cause an abnormally high background signal.
Correct Incorrect
Notes
Load the Plate PHYSICAL INJURY HAZARD. During instrument operation, the
sample block can be heated to 100 °C. Before performing the following procedure, be
sure to wait until the sample block reaches room temperature.
2. Load the plate into the plate holder in the instrument. Ensure that the plate is
properly aligned in the holder.
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3. Close the tray door. Apply pressure to the right side of the tray door at an angle.
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Notes
Start the Run 1. In the 7500 software, select Instrument Instrument Maintenance Manager.
Note: Before starting the run, the instrument may pause (up to 10 min) to allow the
heated cover to reach the correct temperature.
Notes
Verify the Results Note: After the 7500 software completes the RNase P run, it automatically analyzes the
of the Analysis run and displays the results in the Analysis screen.
1. In the Analysis screen of the RNase P Run wizard, verify the status of the run:
• Passed – The 7500/7500 Fast instrument passed the RNase P run. Go to step 5
on page 53.
• Failed – The 7500/7500 Fast instrument failed the RNase P run. Go to step 2 to
review the data for outliers.
If the run fails, the automated analysis may have included outliers that caused the
initial analysis to fail. Experimental error may cause some wells to be amplified
insufficiently or not at all. These wells typically produce CT values that differ
significantly from the average for the associated replicate wells. If included in the
calculations, these outlying data (outliers) can result in erroneous measurements.
2. In the Amplification Plot, select Ct vs. Well from the Plot Type drop-down list.
3. Verify the uniformity of each replicate population on the reaction plate (controls,
standards, and unknowns) by comparing the groupings of CT values:
a. In the plate layout, select the wells containing the 10,000-copy unknown
population (wells rows F, G, and H).
5K-copy Unknown
Population 1
10K-copy Unknown
Population 2
b. In the plot, verify that the CTs of the replicate population are equivalent.
Note: The numbers on the X-axis of the plot correspond to the wells of the
reaction plate. Beginning with well A1, the wells are numbered from
left-to-right, and top-to-bottom.
Notes
7500 System
6 6 0 0
7500 Fast System
IMPORTANT! If the number of outliers exceeds the limit in the table above,
order another RNase P plate and repeat the experiment.
3c 4
2
3a
3b
Outlier
Notes
b. Click the upper-left corner of the Plate Layout to select all wells.
5a
5b
5c
8. Click Finish, then click Yes when prompted to save the experiment.
Notes
More than the • Possible contamination Contact your Applied Biosystems service and sales
maximum number of • Pipetting inaccuracy representative to order a replacement TaqMan® RNase P
outliers are present Instrument Verification Plate. If the replacement RNase P plate
in RNase P data fails, contact Applied Biosystems technical support or your
service representative for further assistance.
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2. Hold the plate up to a light source, and verify that all wells
contain the same volume of fluid.
If there are differences in fluid volumes, check the heat seal
of the wells with lower volumes for signs of damage or
evaporation.
Also, compare the position of the wells that have lower
volumes with the outliers that you have removed from the
plate. If the well positions coincide, the heat seal on the
plate may be defective and resulted in the evaporation of
the associated samples.
3. Contact your Applied Biosystems service and sales
representative to order a replacement TaqMan® RNase P
Instrument Verification Plate. If the replacement RNase P
plate fails, contact Applied Biosystems technical support or
your service representative for further assistance.
Notes
User-Performed Maintenance
Note: For more information about any of the topics discussed in this guide, access the
Help from within Applied Biosystems 7500/7500 Fast Real-Time PCR System Software
v2.0 by pressing F1, clicking in the toolbar, or selecting Help 7500 Software Help.
Notes
Display the 1. In the 7500 software, select Instrument Instrument Events Log.
Instrument Log
2. In the Instrument Events Log dialog box, select either:
• System Log – To view events that occurred during the 25 most recent runs
(experiments) or calibrations.
• Document Log – To view events that pertain only to the experiment currently
open in the 7500 software.
3. If necessary, modify the data displayed by the table by filtering the data and adding
or removing columns.
To… Action
Filter the data in the 1. In the Filter drop-down list, select a property.
events table
2. Enter the appropriate conditions into the drop-down lists
and fields that appear automatically.
3. Click Apply to filter the data.
Note: To reset the log, select Filter Show All Records.
Add or remove columns Click Show Columns, then select the column desired column
to/from the events table in the drop-down list.
Sort the data in the Click the heading of the column of interest once to sort the
events table data in ascending order. Click the column heading again to
sort the data in reverse order.
Export the contents of 1. Select the rows of interest in the event table,
the instrument event
2. Press Ctrl+C to copy the data.
log
3. Paste the data into a spreadsheet application or a text file.
Note: The software exports the data in tab-delimited format.
4. When you finish viewing the events, click the close box to close the dialog box.
Notes
Notes
Check the Lamp In the 7500 software, select Instrument Lamp Status/Replacement to determine the status
Status of the halogen lamp.
Warnings The 7500 software can display the following warnings before or during a run:
Message Description
Warning – Cannot detect sufficient current The lamp current is below the acceptable level at the start of the run. You cannot
from lamp. Either lamp is not installed proceed with the run until you replace the halogen bulb as explained in “Replace
properly or needs to be replaced. the Halogen Lamp” on page 63.
Warning – Cannot detect sufficient current The 7500 software stopped the run because the lamp current decreased below the
from lamp. Either lamp is not installed acceptable level during the run. You cannot proceed with the run until you replace
properly or needs to be replaced. the halogen bulb as explained in “Replace the Halogen Lamp” on page 63. Click
OK in the message box, inspect the Instrument Log, then replace the lamp bulb.
Warning - The lamp usage has exceeded The lamp usage exceeds 2000 hr at the start of a run. Click Cancel Run, then
2000 hr. We recommend replacing the lamp replace the lamp, or click Continue Run.
soon to ensure optimal assay performance.
Rerun ROI, Background, Optical and Dye calibrations.
Notes
Cotton or nylon
swabs and
Pipette (100-µL) lint-free cloths
Powder-free
with pipette tips
gloves
Deionized
water
Clean the IMPORTANT! Wear powder-free gloves when you perform this procedure.
Sample Block
1. Identify the contaminated wells of the sample block (see “How to Identify
Contamination” on page 30).
2. Remove the plate and the tray holder from the 7500/7500 Fast instrument:
a. Push the tray door to open it.
Notes
c. Close the tray door. Apply pressure to the right side of the tray door at an angle.
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3. Manually raise the block:
a. In the 7500 software, select Instrument Instrument Maintenance
Manager.
b. In the ROI tab of the Instrument Maintenance Manager, click Start Manual
Calibration.
c. In the ROI Inspector dialog box, click Move Block.
d. When the ROI Inspector dialog box displays “Block Down,” click Done.
4. Power off, then unplug the 7500/7500 Fast instrument. Allow it to cool for 15 min.
a b
6. Lift the latch, then push the heated cover door to the back of the instrument.
Notes
7. Clean the contaminated wells of the sample block using a small volume of deionized
water:
a. Pipette a small volume of deionized water into each contaminated well.
b. Pipette the water up and down several times to rinse the well.
a d e
8. Pull the heated cover door to the front of the 7500/7500 Fast instrument. Lift the
latch, then secure the heated cover door to the cross bar.
GR2482 GR2482
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heated cover assembly
11. Verify that you have eliminated the contamination by performing a background
calibration run (see “Perform the Background Calibration” on page 20).
Notes
12. If the contamination remains, repeat steps 1 through 6, then clean the contaminated
wells of the sample block using 95% ethanol solution:
a. Pipette a small volume of 95% ethanol solution into each contaminated well.
b. In each contaminated well, pipette the solution up and down several times to
rinse the well.
c. Pipette the ethanol solution to a waste beaker.
IMPORTANT! Always use deionized water to rinse wells after cleaning with bleach
or ethanol solution.
13. Repeat steps 7 through 11 to rinse the wells of the sample block and to verify that
you have eliminated the contamination.
14. If the contamination remains, repeat steps 1 through 6, then clean the contaminated
wells of the sample block using 10% bleach solution:
a. Pipette a small volume of 10% bleach solution into each contaminated well.
b. In each contaminated well, pipette the solution up and down several times to
rinse the well.
c. Pipette the bleach solution to a waste beaker.
IMPORTANT! Always use deionized water to rinse wells after cleaning with bleach
or ethanol solution.
15. Repeat steps 7 through 11 to rinse the wells of the sample block and to verify that
you have eliminated the contamination.
If the contamination remains, contact Applied Biosystems support (see “How to
Obtain Support” on page x).
16. Ensure that the heated cover door is completely closed and latched. If it is not, the
7500 software displays an error message.
Notes
Materials
Required
Replace the IMPORTANT! Wear powder-free gloves when you handle the lamp.
Lamp
1. Power off, then unplug the 7500/7500 Fast system. Allow the instrument to cool for
15 min.
Notes
b. Firmly grasp the lamp and lift it up and out of the slotted mount.
IMPORTANT! Do not touch the lamp without powder-free gloves. Finger prints
shorten the lamp life.
a b
4. Inspect the lamp for signs of failure (carbon typically coats the inside of failed
lamps).
Good bulb
Failed bulb
Replace
b. Firmly grasp the lamp, place it into the slotted mount, then carefully slide the
lamp downward into place.
a b
Notes
10. While the instrument is running, look through grating of the access door and verify
that the lamp is illuminated, then click Done.
Light should be
visible
11. If the lamp is illuminated, select Instrument Lamp Status/Replacement in the 7500
software, click Reset Lamp Timer, then click OK.
If the lamp is not illuminated, the replacement halogen lamp may be defective.
Replace the lamp again. If the second lamp does not illuminate, check the
instrument fuses for failure (see page 66).
12. Perform the following calibrations after replacing the lamp. See:
• Chapter 2, Perform the Regions of Interest (ROI) Calibration
• Chapter 3, Perform the Background Calibration and Optical Calibration
• Chapter 4, Perform the Dye Calibration
• Chapter 5, Verify the Instrument Performance
Notes
Materials
Required
Fuses (2),
12.5 A, 250 V, Flathead Powder-free Safety
5 x 20 mm screwdriver gloves glasses
3. Remove each fuse from its fuse holder and inspect it for damage. Carbon typically
coats the inside of failed fuses.
Good fuse
Failed fuse
Replace
Notes
Note: The voltage and amperage ratings are on the fuse holder.
Note: Fuse failure can result from fluctuations in the supplied power to the instrument.
To prevent further failures, consider installing an electrical protective device, such as a
UPS or other surge protector. For more information about fuses, see the 7500/7500 Fast
Site Preparation Guide.
Notes
Visit the Applied You can obtain 7500 software updates directly from the service section of the
Biosystems Applied Biosystems website. For the latest services and support information for the
Website 7500/7500 Fast instrument:
1. Go to https://www2.appliedbiosystems.com/support/software/
2. In the Software Downloads page, select the appropriate instrument from the
drop-down list.
3. In the Software Downloads page for your instrument, click Updates - Patches.
The website opens the page describing the latest software updates for the 7500 software.
2. Back up all experiment files by creating a copy of the directory that you are using to
store files.
The default directory for experiments is:
D:\Applied Biosystems\7500\experiments
Notes
Note: For more information about any of the topics discussed in this guide, access the
Help from within Applied Biosystems 7500/7500 Fast Real-Time PCR System Software
v2.0 by pressing F1, clicking in the toolbar, or selecting Help 7500 Software Help.
Notes
Materials ABI PRISM® Optical 96-Well Reaction Plate or Optical 96-Well Fast Plate (unused)
Required
3. If you plan to store the 7500/7500 Fast instrument for more than a week or you plan
to move the instrument, load an unused plate into the tray.
Note: The empty plate protects the internal components of the 7500/7500 Fast
instrument during transport or during periods of inactivity lasting more than a week.
GR2471
GR2477
7300/7500
barcode on plate
GR2471
7500
tray top view
Push
GR2477
Notes
IMPORTANT! Moving your Applied Biosystems 7500/7500 Fast Real-Time PCR System
can create subtle changes in the alignment of the instrument optics.
Materials ABI PRISM® Optical 96-Well Reaction Plate and Optical 96-Well Fast Plate (unused)
Required
Prepare the 1. Load the empty reaction plate into the 7500/7500 Fast instrument.
Instrument
2. Using the ROI Inspector, manually raise the sample block:
a. In the 7500 software, select Instrument Instrument Maintenance
Manager.
b. In the ROI tab of the Instrument Maintenance Manager, click Start Manual
Calibration.
c. In the ROI Inspector dialog box, click Block Up.
~
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F1
1
Tab
F2
2
Q
Caps Lock
F3
Shift
3
W
Ctrl
F4
A
4
E
F9
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Z
F5
5
R
D
X
F6
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T
Alt
F
C
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G
V
F8
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F10
K
_
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-
P
F11
L
<
+=
[
F12
>
"
Print
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? /
Alt
Scroll
Screen Lock
SysRq
Enter
Shift
Pause
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Break
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End
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num
lock
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Down
Num
caps
Lock
lock
7
scroll
4
lock
8
*
1
5
9
0
2
+
6
3 Enter
(120 lbs).
People Lift
Notes
6. Reconnect the components of the 7500/7500 Fast system (see “Set Up the
7500/7500 Fast System” on page 73).
Notes
Set Up the IMPORTANT! Do not connect the USB cable to the 7500/7500 Fast instrument until you are
7500/7500 Fast instructed to do so by this guide.
Instrument
Materials Required
• Phillips screwdriver (small and thin)
• Power cord
1. Prepare the installation site as described in the Applied Biosystems 7500/7500 Fast
Real-Time PCR System Site Preparation Guide.
3. Verify that the heated cover assembly is pulled fully toward the front of the
instrument. If the 7500/7500 Fast system has a heated cover latch installed, check
that the latch is in a locked position.
4. Inspect the instrument for damage caused by the transportation of the 7500/7500
Fast system.
If the instrument is damaged, record the location and appearance of the damage,
then contact Applied Biosystems technical support or your service representative for
assistance.
6. Connect the power cord to the 7500/7500 Fast instrument, then to the wall
receptacle.
Note: Power cords for different voltages are provided in the packing kit. Connect
the cord with the receptacle appropriate for your voltage, then discard the remaining
power cords.
7. Press the power button at the lower right front panel, then wait for the 7500/7500
Fast instrument to start up (about 30 sec).
Notes
8. When the Power status light on the lower left front panel is lit, push the tray door to
open it.
9. Remove the packaging plate from the tray and set it aside.
10. Close the tray door, then press the power button again to power off the instrument.
IMPORTANT! Do not connect the USB cable to the 7500/7500 Fast instrument at
this time.
12. Once you verify that the computer contains the 7500 software, connect the USB
cable to the 7500/7500 Fast instrument.
Notes
The Applied Biosystems 7500/7500 Fast Real-Time PCR System can be used to run
assays designed with custom dyes (dyes not manufactured by Applied Biosystems).
Custom dyes must fluoresce within the 520 to 650 nm spectral range measured by the
7500/7500 Fast instrument.
Before Using Before using custom dyes with the 7500/7500 Fast instrument, you must:
Custom Dyes • Determine optimum dye concentration
• Create a custom dye plate
• Add the custom dye to the software
• Perform a dye calibration (see Chapter 4, “Perform the Dye Calibration.”)
GR2170
Notes
Determine IMPORTANT! Wear powder-free gloves while creating the dye plate.
Optimum Dye
Concentration
1. In the center wells of a 96-well plate, prepare a dilution series of the custom dye (for
example, 25, 50, 100, 200, 400, 800, 1600, and 3200 nM) using 50-µL volumes for
the 7500 system or 20-µL volumes for the 7500 Fast system.
25 50 100 200
2. Seal the wells of the reaction plate using an optical adhesive cover.
GR2471
GR2477
7300/7500
barcode on plate
GR2471
7500
tray top view
Push
GR2477
5. In the ROI tab of the Instrument Maintenance Manager, click Start Manual
Calibration.
6. In the ROI Inspector, create the ROI image for each filter, beginning with Filter 1:
a. In the Exposure Time field, enter 1024.
c. Select Filter 1.
d. Click Snapshot.
Notes
Normal Over
No Saturation
Saturation Saturation
f. Record the coordinate of the well that displays the brightest possible signal
without saturation. This well contains the optimal concentration of the custom
dye for Filter 1.
8. After you determine the optimum concentration for each filter, determine the
optimum concentration for the custom dye:
a. Compare the results from all filters.
b. Select the concentration that yields the highest possible signal in all filters, but
does not saturate.
Notes
Unload the Plate PHYSICAL INJURY HAZARD. During instrument operation, the
sample block can be heated to 100 °C. Before performing the following procedure, be
sure to wait until the sample block reaches room temperature.
Note: If you cannot open the tray, the sample block may be in its raised position, locking
the tray position. To lower the block, click Move Down, then click Block Down.
3. Click Done.
Create a Custom IMPORTANT! Wear powder-free gloves while creating the dye plate.
Dye Plate
1. Prepare 5 mL (7500 system) or 2 mL (7500 Fast system) of the custom dye at the
concentration determined in step 8 on page 77.
2. Pipette 50 µL (7500 system) or 20 µL (7500 Fast system) of the diluted custom dye
to all wells of an optical reaction plate.
3. Seal the wells of the reaction plate using an optical adhesive cover.
IMPORTANT! The custom dye calibration plate must be well mixed and centrifuged.
Notes
5. Verify that the liquid in each well of the ROI calibration plate is at the bottom of the
well. If not, centrifuge the plate again at a higher rpm and for a longer period of time.
Correct Incorrect
Add the Custom 1. In the main screen of the 7500 software, select Instrument
Dye to the Instrument Maintenance Manager.
Software
2. In the Instrument Maintenance Manager:
a. In the navigation pane, click Dye.
3. In the Setup screen of the Dye Calibration dialog box, select a custom dye from the
list or create the custom dye as follows:
a. Click New Dye.
Field/Option Action
Type Select:
• Reporter if the dye works in conjunction with a quencher dye
to report an increase of PCR product.
• Quencher if the dye suppresses the fluorescence of a reporter
dye until amplification of PCR product.
• Both if the dye reports an increase of PCR product without the
aid of a quencher dye.
d. Click Close.
Notes
4. In the Setup screen of the Dye Calibration dialog box, enter a temperature setting for
the calibration.
Note: Set the temperature to match the temperature at which you intend to collect
data. For example, the temperature for all Applied Biosystems system dyes is 60 °C
because data collection for TaqMan® reagents occurs during the 60 °C extension
step of the PCR.
5. Select The custom dye plate is loaded in the instrument, then click Next.
6. In the Run screen, click Start Run, then wait for the 7500/7500 Fast instrument to
complete the dye calibration.
Note: If the 7500 software displays messages during the run, troubleshoot the errors
as described in “Troubleshoot the Dye Calibration” on page 43.
7. When the 7500/7500 Fast instrument displays the Main Menu, unload the custom
calibration plate.
Notes
Whenever possible, use a background plate that is included with the spectral calibration
kit. The plates supplied in the kit contain a buffer that accurately simulates the reagents
used for PCR, and, therefore, produces high-quality calibration data. However, if a
background plate from a spectral calibration kit is not available, you can create one as
described below.
Create a IMPORTANT! Wear powder-free gloves while creating the background plate.
Background Plate
1. Remove an Applied Biosystems 96-Well Optical Reaction Plate or 96-Well Fast
Reaction Plate from its box and place it on a clean, dry surface.
3. Seal the plate using an optical adhesive cover or optical flat caps.
Use the plate for background calibration in the same way you use a background
plate from the spectral calibration kit. See Chapter 3, “Perform the Background
Calibration and Optical Calibration,”
Notes
Notes
A background plate 81
custom dye plate 75–80
access door, open 63
custom dye
analyze add to the software 79
background calibration 23 calibration 79–80
dye calibration 39–42 plate, how to create 75–80
optical calibration 28
RNase P experiment 51–53 CY3® dye 33, 41
ROI calibration (automated) 12 CY5® dye 33, 42
ROI calibration (manual) 13–15
Applied Biosystems D
contacting x
DANGER, description xii
Technical Support x
decontamination
assumptions for using this guide vii
clean the sample block 59–62
identify contaminants 30
B materials required 59
background calibration 20–24 documentation, related viii
analyze the data 23 dye calibration
materials required 20 analyze the data 39–42
perform 23 materials required 32
preparation 21 perform 36
troubleshoot 30 preparation 35
background fluorescence 20 spectra evaluation 34
background plate spectra, 7500 41
troubleshoot 43
how to create 81
prepare 21
biohazardous waste, handling xix E
biological hazard guidelines xxi electrical safety xx
electromagnetic compatibility standards.
C See EMC standards
EMC standards xxii
calibration
background 20–24 ergonomics, safety xxi
dye 32–42
dye (custom) 75–80 F
optical 25–29
ROI 8–17 FAM™ dye 33, 41, 46
CAUTION, description xii Fast plate
description 9
CCD function test 57
do not vortex 9
chemical safety xvii, xviii Filter Wheel function test 57
chemical waste safety xix fluorescence, background 20
conventions
function tests 57
for describing menu commands vii
IMPORTANTS! vii fuse replacement 66–67
Notes vii materials required 66
safety xii
text vii G
user attention words vii
guidelines
create chemical safety xviii
R installation 47
instrument fuses 66
R2 value 53
spectra
radioactive waste, handling xix CY3® dye 41
remove outliers from RNase P runs 51 CY5® dye 42
repetitive motion, safety xxi FAM™ dye 41
replace JOE™ dye 41
halogen lamp 63–65 NED™ dye 41
instrument fuses 66–67 ROX™ dye 42
reset lamp timer 58 SYBR® Green I dsDNA Binding dye 41
TAMRA™ dye 41
RNase P experiment 46–53
TEXAS RED® dye 42
analyze 51–53
VIC® dye 41
materials required 46
perform 49 standard plate, description 9
preparation 48 standards
prepare 48 EMC xxii
R2 value 53 safety xxii
troubleshoot 54 storage, prepare instrument for inactivity 70
ROI calibration 8–17 SYBR® Green I dsDNA Binding dye 33, 41
analyze the data (automated) 12 symbols, safety xiii
analyze the data (manual) 13–15 system dye
materials required 8 CY3® dye 33, 41
perform 12 CY5® dye 33, 42
preparation 9 FAM™ dye 33, 41, 46
saturation examples 13 JOE™ dye 33, 41
successful 14 NED™ dye 33, 41
troubleshoot 17 ROX™ dye 33, 42
ROX™ dye 33, 42 SYBR® Green I dsDNA Binding dye 33, 41
TAMRA™ dye 33, 41
S TEXAS RED® dye 33, 42
VIC® dye 33, 41
safety
before operating the instrument xvi
biological hazards xxi T
chemical xvii TAMRA™ dye 33, 41
chemical waste xix TaqMan® Fast Universal PCR Master Mix, No
conventions xii AmpErase® UNG 46
electrical xx
ergonomic xxi Technical Support, contacting x
guidelines xviii, xix TEXAS RED® dye 33, 42
instrument operation xvi Thermal Cycler function test 57
moving and lifting instrument xvi training, information on x
moving parts xx troubleshoot
moving/lifting xvi background calibration 30
physical hazard xx dye calibration 43
repetitive motion xxi function tests 57
standards xxii instrument fuses 66–67
workstation xxi instrument log 56
safety labels, on instruments xiv lamp replacement 63–65
safety standards xxii lamp status, view 58
safety symbols, on instruments xiii optical calibration 30
saturation, ROI calibration 13 RNase P experiment 54
ROI calibration 17
service pack, updates 67 sample block decontamination 59
set up, instrument (after storage or transport) 73
Shutter function test 57
U
specification
halogen lamp 63 update
operating system 67
service packs 67
USB function test 57
user attention words, described vii
V
VIC® dye 33, 41
W
WARNING, description xii
waste disposal, guidelines xix
workstation safety xxi
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06/2010