Fast MicroSeq D2 LSU rdna Fungal Identification Kit

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1 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

2 Copyright 2007, 2010 Applied Biosystems. All rights reserved. For Research Use Only. Not for use in diagnostic procedures. Information in this document is subject to change without notice. Applied Biosystems assumes no responsibility for any errors that may appear in this document. In no event shall Applied Biosystems be liable for incidental, special, multiple, or consequential damages in connection with or arising from the use of this document. NOTICE TO PURCHASER: LIMITED LICENSE for the Fast MicroSeq D2 LSU rdna Fungal PCR Kit (PN ) Use of this product is covered by US patent claims and corresponding patent claims outside the US. The purchase of this product includes a limited, non-transferable immunity from suit under the foregoing patent claims for using only this amount of product solely in the environmental testing, quality control/quality assurance testing, food and agricultural testing applications, including reporting results of purchaser s activities for a fee or other commercial consideration, and also for the purchaser's own internal research. No right under any other patent claim (such as the patented 5 Nuclease Process claims), is conveyed expressly, by implication, or by estoppel. Further information on purchasing licenses may be obtained by contacting the Director of Licensing, Applied Biosystems, 850 Lincoln Centre Drive, Foster City, California 94404, USA. NOTICE TO PURCHASER: LIMITED LICENSE for the MicroSeq D2 LSU rdna Fungal Sequencing Kit (PN ) A license under the process claims of U.S. patent claims or their foreign counterpart claims, has an up-front fee component and a running-royalty component. The purchase price of the MicroSeq D2 LSU rdna Fungal Sequencing Kit includes limited, nontransferable rights under the running-royalty component to use only this amount of the product to practice the DNA sequence and fragment analysis processes described in said patents when this product is used in conjunction with an Authorized DNA sequence analysis instrument whose use is covered under the up-front fee component of these patents. No other rights are hereby granted expressly, by implication, or by estoppel, or under any other patent rights owned or licensable by Applied Biosystems. Further information relating to the purchase of licenses for DNA sequence and fragment analysis and other applications may be obtained by contacting the Director of Licensing at Applied Biosystems, 850 Lincoln Centre Drive, Foster City, CA 94404, USA. NOTICE TO PURCHASER: LIMITED LICENSE The purchase of the MicroSeq D2 LSU rdna Fungal Sequencing Kit includes a limited, nontransferable, non-exclusive license (without the right to resell, repackage, or sublicense) under US patent claims, and corresponding foreign patent claims and patent applications, to use this product solely with an Applied Biosystems commercial automated DNA sequencing machine or other authorized automated DNA sequencing machine that has been authorized under these patents by Applied Biosystems. No license is hereby granted for the use of this kit or the reagents therein, in any other automated sequencing machine. Such license is granted solely for research and other uses that are not unlawful. No other license is granted expressly, impliedly, or by estoppel. Further information on purchasing licenses may be obtained by contacting the Director of Licensing, Applied Biosystems, 850 Lincoln Centre Drive, Foster City, California 94404, USA. NOTICE TO PURCHASER ABOUT LIMITED LICENSE This kit (reagent) is sold pursuant to a limited sublicense from Amersham International plc under one or more U.S. Patent Nos. 5,498,523; 5,614,365, and corresponding foreign patents and patent applications. The purchase of this kit (reagent) includes a limited non-exclusive sublicense (without the right to resell, repackage or further sublicense) under such patent rights to use this reagent for DNA sequencing or fragment length analysis solely with an Applied Biosystems commercial automated sequencing machine or other authorized DNA sequencing machines that have been authorized for such use by Applied Biosystems, or for manual DNA sequencing. No license is hereby granted for use of this kit, or the reagents therein, in any other automated sequencing machine. Such sublicense is granted solely for research or other uses that are not unlawful. No other license is granted expressly, implied, or by estoppel. For information concerning the availability of additional license to practice the patented methodologies, contact: Amersham Life Science, Inc., Vice President, Regulatory Affairs, P.O. Box 22400, Cleveland, Ohio Patents are pending in countries outside the United States. TRADEMARKS: AB (Design), ABI PRISM, Applera, Applied Biosystems, BigDye, GeneAmp, MicroAmp, MicroSeq, and PrepMan are registered trademarks and Hi- Di, and MicroAmp are trademarks of Applied Biosystems or its subsidiaries in the U.S. and/or certain other countries. All other trademarks are the sole property of their respective owners. Part Number Rev. B Printed 06/2010

3 Contents Preface v Purpose v Audience v Safety v How to Obtain Services and Support ix Related Documentation x Introduction MicroSeq System Overview Fast MicroSeq Product Description About Dye Terminator Chemistry Instrument Platforms Protocol Overview PCR Good Laboratory Practices Materials and Equipment Kit Contents Storage Guidelines Equipment and Materials Not Included Isolating DNA PrepMan Ultra Sample Preparation Reagent Storing the DNA Sample Preparing the Working Stock of Fungal Genomic DNA Performing PCR Minimizing the Effects of PCR Inhibition Performing PCR Analyzing PCR Products (Optional) Purifying PCR Products for Cycle Sequencing Performing Cycle Sequencing Preparing Cycle Sequencing Reactions Performing Cycle Sequencing Purifying Extension Products Performing Electrophoresis of Extension Products Configuring the Instrument for Electrophoresis Performing the Run Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol iii

4 Analyzing Data MicroSeq ID Analysis Software MicroSeq Proprietary Libraries Custom Libraries MicroSeq Reports Troubleshooting Frequently Asked Questions Running 30 Cycles Instead of 35 Cycles Sensitivity and Quantification Sample Preparation and Storage Contamination Overlapping Sequences PCR Product Size Species Libraries Additional Documentation Appendix A, Fast MicroSeq D2 LSU rdna Fungal Identification Products Appendix B, Additional Supported Applied Biosystems Instruments Materials Instrument Configurations for Electrophoresis References Index iv Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

5 Preface This preface contains: Purpose v Audience v Safety v How to Obtain Services and Support ix Related Documentation x Purpose Audience Safety The purpose of this protocol is to simplify the steps of DNA isolation, PCR, cycle sequencing, electrophoresis, and data analysis. The protocol assumes some experience with PCR techniques. The protocol is written for users of the Applied Biosystems Fast MicroSeq D2 LSU rdna Fungal PCR and MicroSeq D2 LSU rdna Fungal Sequencing Kits. Safety Alert Words Four safety alert words appear in Applied Biosystems user documentation at points in the document where you need to be aware of relevant hazards. Each alert word IMPORTANT, CAUTION, WARNING, DANGER implies a particular level of observation or action, as defined below: IMPORTANT! Indicates information that is necessary for proper instrument operation, accurate chemistry kit use, or safe use of a chemical. Indicates a potentially hazardous situation that, if not avoided, may result in minor or moderate injury. It may also be used to alert against unsafe practices. Indicates a potentially hazardous situation that, if not avoided, could result in death or serious injury. Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol v

6 Indicates an imminently hazardous situation that, if not avoided, will result in death or serious injury. This signal word is to be limited to the most extreme situations. Chemical Hazard Warning CHEMICAL HAZARD. Some of the chemicals provided in your reagent kit may be hazardous. Before handling the reagents, read the material safety data sheets (MSDSs) that accompany your first shipment. Always follow the safety precautions outlined in each MSDS. "Obtaining MSDSs" section below describes how you can receive additional copies of of MSDS at no extra cost. CHEMICAL HAZARD. Some of the chemicals used in this protocol are hazardous. Follow the safety precautions stated in the specific chemical warnings that appear throughout this protocol. CHEMICAL HAZARD. Some of the chemicals referred to in this protocol may not have been provided with your kit. If the chemicals are not provided, they are not manufactured or sold by Applied Biosystems. Please obtain the MSDSs from their manufacturers. Chemical Safety Guidelines To minimize the hazards of chemicals: Read and understand the Material Safety Data Sheets (MSDS) provided by the chemical manufacturer before you store, handle, or work with any chemicals or hazardous materials. (See About MSDSs. ) Minimize contact with chemicals. Wear appropriate personal protective equipment when handling chemicals (for example, safety glasses, gloves, or protective clothing). For additional safety guidelines, consult the MSDS. Minimize the inhalation of chemicals. Do not leave chemical containers open. Use only with adequate ventilation (for example, fume hood). For additional safety guidelines, consult the MSDS. vi Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

7 Check regularly for chemical leaks or spills. If a leak or spill occurs, follow the manufacturer s cleanup procedures as recommended on the MSDS. Comply with all local, state/provincial, or national laws and regulations related to chemical storage, handling, and disposal. 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 You can obtain from Applied Biosystems the MSDS for any chemical supplied by Applied Biosystems. This service is free and available 24 hours a day. To obtain MSDSs: 1. Go to 2. In the Search field, type in the chemical name, 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 Chemical Waste Hazard CHEMICAL WASTE HAZARD. Some wastes produced by the operation of the instrument or system are potentially hazardous and can cause injury, illness, or death. Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol vii

8 Chemical Waste Safety Guidelines To minimize the hazards of chemical waste: Read and understand the Material Safety Data Sheets (MSDSs) provided by the manufacturers of the chemicals in the waste container before you store, handle, or dispose of chemical waste. Provide primary and secondary waste containers. (A primary waste container holds the immediate waste. A secondary container contains spills or leaks from the primary container. Both containers must be compatible with the waste material and meet federal, state, and local requirements for container storage.) Minimize contact with chemicals. Wear appropriate personal protective equipment when handling chemicals (for example, safety glasses, gloves, or protective clothing). For additional safety guidelines, consult the MSDS. Minimize the inhalation of chemicals. Do not leave chemical containers open. Use only with adequate ventilation (for example, fume hood).for additional safety guidelines, consult the MSDS. Handle chemical wastes in a fume hood. After emptying the waste container, seal it with the cap provided. Dispose of the contents of the waste tray and waste bottle in accordance with good laboratory practices and local, state/provincial, or national environmental and health regulations. 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. IMPORTANT! Biohazardous materials may require special handling, and disposal limitations may apply. viii Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

9 Biological Hazard Safety BIOHAZARD. Biological samples such as tissues, body fluids, and blood of humans and other animals have the potential to transmit infectious diseases. Follow all applicable local, state/provincial, and/or national regulations. Wear appropriate protective eyewear, clothing, and gloves. Read and follow the guidelines in these publications: U.S. Department of Health and Human Services guidelines published in Biosafety in Microbiological and Biomedical Laboratories (stock no ; Occupational Safety and Health Standards, Bloodborne Pathogens (29 CFR ; waisidx_01/29cfr1910a_01.html) Additional information about biohazard guidelines is available at: How to Obtain Services and Support Related Documentation For the latest services and support information for all locations, go to then click the link for Support. At the Services and Support page, you can: Obtain worldwide telephone and fax numbers to contact Applied Biosystems Technical Support and Sales facilities Search through frequently asked questions (FAQs) Submit a question directly to Technical Support Order Applied Biosystems user documents, MSDSs, certificates of analysis, and other related documents Download PDF documents Obtain information about customer training Download software updates and patches Information about the MicroSeq ID Analysis Software is available in the: MicroSeq ID Analysis Software Version 2.0 Quick Reference Card (PN ) MicroSeq ID Analysis Software Version 2.0 Getting Started Guide (PN ) Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol ix

10 MicroSeq ID Analysis Software Version 2.0 Online Help Applied Biosystems MicroSeq web site at x Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

11 Introduction Introduction MicroSeq System Overview Fast MicroSeq Product Description The MicroSeq Microbial Identification System combines the advantages of reagents for bacterial and fungal PCR and sequencing, MicroSeq ID Analysis Software, easy PrepMan Ultra Sample Preparation Reagent, robust protocols, and state-of-the-art thermal cyclers and sequencing instruments. The MicroSeq system is easy to use and suitable for the routine identification of all bacterial and fungal isolates, including organisms that are difficult to grow, non-viable, or unidentifiable using phenotypic methods. The MicroSeq system identifies bacterial and fungal isolates from a small sample of pure culture without preliminary testing or growth on selective media. The Fast MicroSeq D2 LSU rdna Identification Kit consists of the Fast MicroSeq D2 LSU rdna Fungal PCR Kit and the MicroSeq D2 LSU rdna Fungal Sequencing Kit. These kits provide all the reagents necessary for the amplification and sequencing of the D2 region of the nuclear large-subunit (LSU) ribosomal RNA gene. The DNA sequence of the gene is then determined through the process of capillary electrophoresis on an Applied Biosystems genetic analyzer. Using MicroSeq ID Analysis Software, the sequence is compared to a MicroSeq Fungal Gene library that contains D2 sequence entries from more than 1000 validated species, then an identification report is generated. Variations found within the D2 region are sufficient to identify most yeast and molds to the species level. Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 1

12 About Dye Terminator Chemistry The MicroSeq D2 LSU rdna Fungal Sequencing Kit uses Applied Biosystems BigDye Terminator v1.1 chemistry. The Forward and Reverse Sequencing Mixes are part of the sequencing dye-labeled 3 - dideoxynucleotide triphosphates (dye terminators). With dye terminator labeling, each of the four dideoxy terminators (ddntps) is tagged with a different fluorescent dye. When dyelabeled terminators are in the reaction mix, extension products are simultaneously terminated and labeled with the dye that corresponds to the incorporated base, as shown in the following figure. For more information about dye terminator and other sequencing chemistries, refer to the ABI PRISM Automated DNA Sequencing Chemistry Guide (PN ). Instrument Platforms For optimum performance of the Fast MicroSeq D2 LSU rdna Fungal Identification Kit, use the: Applied Biosystems 9800 Fast Thermal Cycler Applied Biosystems 3130 and 3130xl Genetic Analyzers Note: You can use a GeneAmp PCR System 9700 instead of a 9800 Fast Thermal Cycler, but the 9700 does not provide the short amplification and sequencing times allowed by the new FAST Microseq D2 PCR chemistry and the 9800 Fast Thermal Cycler. For information on older instruments that can also be used, see Appendix B, Additional Supported Applied Biosystems Instruments on page Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

13 F1 F2 F3 F4 F STOP GeneAmp PCR System 9700 ENTER 0 CE F1 F2 F3 F4 F STOP GeneAmp PCR System 9700 ENTER 0 CE POWER POWER Introduction Protocol Overview This protocol provides: A list of materials and equipment required to determine the sequence of the D2 expansion segment region of the LSU ribosomal RNA gene Instructions for performing PCR and cycle sequencing, and for purifying PCR and extension products Information about interpreting results Workflow Procedure Harvest Yeast or Filamentous Fungal Colony Isolate DNA, make working stock of DNA, then prepare for PCR Perform PCR, then analyze and purify PCR products Applied Biosystems 9800 Fast Thermal Cycler Perform Cycle Sequencing, then purify extension products Applied Biosystems 9800 Fast Thermal Cycler Perform Electrophoresis Applied Biosystems 3130/3130xl Genetic Analyzer Analyze Data MicroSeq ID Analysis Software Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 3

14 PCR Good Laboratory Practices PCR assays require special laboratory practices to avoid false positive amplifications (Kwok and Higuchi, 1989). The high throughput and repetition of these assays can lead to amplification of a single DNA molecule (Saiki et al., 1985; Mullis and Faloona, 1987). Wear a clean lab coat (not previously worn while handling amplified PCR products or used during sample preparation) and clean gloves when preparing samples for PCR amplification. Change gloves whenever you suspect that they are contaminated. Maintain separate areas, dedicated equipment, and supplies for: Sample preparation and PCR setup PCR amplification and post-pcr analysis Never bring amplified PCR products into the PCR setup area. Open and close all sample tubes carefully. Do not splash or spray PCR samples. Quick-spin PCR samples whenever residual sample is present on the inside lid (such as after dropping a tube or when there is condensation on the tube from heating or thawing). Keep reactions and components capped as much as possible. Use positive-displacement pipettes or aerosol-resistant pipette tips. Clean lab benches and equipment periodically with freshly diluted 10% bleach solution. Clean the PCR set-up area with DNAZap TM reagent (Ambion NP AM9890). 4 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

15 Materials and Equipment Materials and Equipment Kit Contents The tables below describe the contents of the two fungal kits. Fast MicroSeq D2 LSU rdna Fungal PCR Kit (PN ) Component Fast MicroSeq D2 LSU rdna Fungal PCR Master Mix Fast MicroSeq D2 LSU rdna Fungal PCR Primer Mix Positive Control DNA Negative Control (Water) Description One tube (with yellow cap) containing PCR Master Mix sufficient for 60 PCR amplifications One tube (with red cap) containing PCR primers specific to D2 region of LSU rrna gene from fungal genomic DNA. One tube of positive control DNA (S. cerevisiae) at 1 ng/µl, sufficient for 10 positive-control assays One tube of negative control The MicroSeq D2 LSU rdna Fungal Sequencing Kit (PN ) Component D2 Forward Sequencing Mixes D2 Reverse Sequencing Mix Description Two tubes containing enough mix to perform a total of 55 reactions Two tubes containing enough mix to perform a total of 55 reactions Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 5

16 Storage Guidelines Kit Storage Kit On Receipt Storage Conditions After First Use PCR 15 to 25 C 2 to 8 C in a PCR clean room Sequencing 15 to 25 C 15 to 25 C Avoid excess freeze-thaw cycles. Aliquot reagents in smaller amounts, if necessary. Before each use of the kit, allow the frozen stocks to thaw at room temperature. IMPORTANT! Do not heat the reagents. Whenever possible, keep thawed materials on ice during use. Mix the contents of each tube by gently vortexing the tubes. Centrifuge the tubes briefly to collect all liquid at the bottom of the tube. Equipment and Materials Not Included The items in the following two tables are required in addition to the reagents supplied in the Fast MicroSeq D2 LSU rdna Fungal Identification Kit. Instruments Instrument Applied Biosystems 3130/3130xl Genetic Analyzer Applied Biosystems 9800 Fast Thermal Cycler Note: You can use a GeneAmp PCR System 9700, but the PCR and sequencing steps require more time. Source Contact your local Applied Biosystems sales office. For information on older instruments that you can also use, see Appendix B, Additional Supported Applied Biosystems Instruments on page Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

17 Materials and Equipment User-supplied materials Materials Source 3100/3130 BigDye Terminator v1.1 Sequencing Standard (310, 3100, 3100-Avant, 3130, and 3130xl instruments) For the Applied Biosystems 9800 Fast Thermal Cycler To use FAST 96-well plates on a 3100/3130 Genetic Analyzer Applied Biosystems (PN ) xl FAST plate adapter kit Applied Biosystems (PN ) To run MicroSeq kit reagents in 96-well plates Optical 96-Well Fast Thermal Cycling Plate with Barcode Applied Biosystems (PN ) MicroAmp Clear adhesive film Applied Biosystems (PN ) MicroAmp Caps, 8 Caps/Strip or 12 Caps/Strip Applied Biosystems (PN N or N ) MicroAmp Cap Installing Tool Applied Biosystems (PN ) MicroAmp adhesive film applicator Applied Biosystems (PN ) MicroAmp optical film compression pad Applied Biosystems (PN ) MicroAmp Splash Free 96-Well Base Applied Biosystems (PN ) To run MicroSeq kit reagents in MicroAmp tubes Fast Reaction Tubes, 0.1-mL Applied Biosystems (PN ) Fast 96-Well Retainer Tray Applied Biosystems (PN ) MicroAmp Splash Free Support Base or MicroAmp Splash Free 96-Well Base MicroAmp Caps, 8 Caps/Strip or 12 Caps/Strip Applied Biosystems (PN or N ) Applied Biosystems (PN N or N ) MicroAmp Cap Installing Tool Applied Biosystems (PN ) For Applied Biosystems GeneAmp PCR System 9700 To run MicroSeq kit reagents in 96-well plates Optical 96-Well Optical Reaction Plate Applied Biosystems (PN ) MicroAmp clear adhesive film Applied Biosystems (PN ) MicroAmp Caps, 8 Caps/Strip or 12 Caps/Strip Applied Biosystems (PN N or N ) MicroAmp Cap Installing Tool (Handle) Applied Biosystems (PN ) Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 7

18 User-supplied materials (continued) Materials Source MicroAmp adhesive film applicator Applied Biosystems (PN ) MicroAmp optical film compression pad Applied Biosystems (PN ) MicroAmp Splash Free 96-Well Base Applied Biosystems (PN ) To run MicroSeq kit reagents in MicroAmp tubes MicroAmp 96-Well Support Base or MicroAmp Splash Free 96-Well Base Applied Biosystems (PN N or ) 96-Well Tray/Retainer Set Applied Biosystems (PN ) MicroAmp Cap Installing Tool (Handle) Applied Biosystems (PN ) MicroAmp Reaction Tubes, 0.2-mL or MicroAmp 8-tube strip, 0.2-mL MicroAmp Caps, 8 Caps/Strip or 12 Caps/Strip Applied Biosystems (PN N or N ) Applied Biosystems (PN N or N ) PrepMan Ultra Sample Preparation Reagent Applied Biosystems (PN ) Nuclease-Free Water (not DEPC treated) No-Stick, RNase-Free 1.5-mL microfuge tubes Table-top centrifuge, with 96-tube tray adapter Fixed-angle microcentrifuge FlashGel System as needed: Ambion (PN AM9937) Ambion (PN AM12450) Eppendorf (5804) or equivalent Eppendorf (5415D) or equivalent Cambrex FlashGel Starter Pack FlashGel Dock FlashGel Casette ExoSAP-IT Reagent USB (78200) Montage PCR Filter Unit Millipore (UFC7 PCR 50) Extension purification product as needed CentriSep Spin Column Applied Biosystems (PN ) DyeEx 96 Kit Qiagen (PN 63181) DyeEx 2.0 Spin Kit Qiagen (PN 63204) Performa DTR Gel Filtration Cartridges Edge Biosystems (PN 98780) Performa DTR Ultra 96-Well Plate Kit Edge Biosystems (PN 54789) Hi-Di formamide Applied Biosystems (PN ) 8 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

19 Materials and Equipment User-supplied materials (continued) Materials Source Vortexer Major Laboratory Supplier (MLS). BigDye Terminator Sequencing Standards are required for spectral calibration of the sequencing instrument with Big Dye Terminator v1.1, and for verifcation of instrument performance. Refer to the instrument manual for additional information.. United States Biochemical. Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 9

20 Isolating DNA PrepMan Ultra Sample Preparation Reagent Storing the DNA Sample Preparing the Working Stock of Fungal Genomic DNA PrepMan Ultra Sample Preparation Regeant contains a material that may cause eye, skin, and respiratory tract irritation, and adverse effects on the kidneys and blood and central nervous system. Read the MSDS, and follow the handling instructions. Wear appropriate protective eyewear, clothing, and gloves. Isolate fungal genomic DNA using Applied Biosystems PrepMan Ultra sample preparation reagent (PN ). Follow the instructions in the PrepMan Ultra Sample Preparation Reagent Protocol (PN ). IMPORTANT! The ideal colony size is 2 to 3 mm. For smaller colonies, decrease the amount of PrepMan Ultra sample reagent to 50 µl from the suggested 100 µl in the protocol. For additional information on isolating genomic DNA, go to At the end of the PrepMan Ultra procedure, the supernatant contains fungal genomic DNA that can be stored at 20 C indefinitely, or at 4 C for up to 1 month. Dilute the PrepMan Ultra supernatant in water as described below. 1. Pipette 495 µl of nuclease-free water (AM9937) into a 1.5-mL microcentrifuge tube (AM12450). 2. Add 5 µl of the PrepMan Ultra supernatant to get a 1:100 dilution. For samples with low biomass, make a smaller dilution (for example, use 195 µl of nuclease-free water to make a 1:40 dilution). 3. Vortex the tube to mix the solution. 4. Store the remaining supernatant at 20 C. 10 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

21 Performing PCR Performing PCR Minimizing the Effects of PCR Inhibition Inhibitors of PCR in the working stock of fungal DNA can interfere with amplification of the desired region of the rrna gene. If the PrepMan Ultra supernatant is colored (typically blackish or greenish), PCR inhibition is likely to occur. One way to avoid PCR inhibition is to further dilute your working stock of fungal genomic DNA before PCR. For example, add 45 µl of nuclease-free water to 5 µl of your working stock to make a 1:1000 dilution of your original PrepMan Ultra supernatant. Making several dilutions of each sample and performing PCR for each of them increases your chances of obtaining a PCR product of the correct size. If you do not obtain a PCR product from any of the diluted samples, use a DNA extraction kit to isolate pure DNA. Alternatively, you can try the bead-beating method described at Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 11

22 Performing PCR New FAST Microseq D2 PCR chemistry consists of two components: FAST MicroSeq D2 LSU rdna Fungal PCR Master Mix (tube with yellow cap) FAST MicroSeq D2 LSU rdna Fungal PCR Primer Mix (tube with red cap) 1. a. b. Prepare D2 reaction mix: In a single tube combine 14 µl of the PCR Master Mix and 2 µl of the PCR Primer Mix for each sample or control. Vortex briefly, then spin down to collect all liquid at the bottom of the tube. Dispense as described in step Prepare samples and controls in tubes or 96-well plates appropriate for your thermal cycler (see page 7). To prepare... Combine... Negative controls 15 µl of D2 Reaction Mix 15 µl of negative-control water Positive controls 15 µl D2 Reaction Mix 15 µl of positive-control DNA Samples 15 µl of D2 Reaction Mix 15 µl working stock (1:100 dilution of PrepMan Ultra supernatant) 3. Cap the tubes or seal the 96-well plate with the 96-well heat seal, then place in the thermal cycler. 12 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

23 Performing PCR 4. Use the following conditions for the 9800 Fast Thermal Cycler. Note: You can use the same conditions for a 9700 thermal cycler in a Max mode, but the cycle can take up to 20 minutes longer. Initial Step Each of 35 Cycles Final Extension Final Step Melt Anneal HOLD CYCLE HOLD HOLD 95 C 10 sec 95 C 0 sec 64 C 15 sec 72 C 1 min 4 C 5. Set the reaction volume for thermal cycling to 30 µl. 6. Start the run. 7. Store the PCR products at 15 to 25 C until you are ready to use them. PCR products are stable for at least 6 months or longer at 20 C. Analyzing PCR Products (Optional) Determine if a PCR product is in your samples by running a 1.2% agarose gel separation (Cambrex FlashGel cassette 57023). Load 5 µl of the PCR product per lane to detect amplified DNA. Use the Mass Standard Ladder to estimate the PCR product yield. The sequencing protocol works best with 5 to 20 ng of amplicon input. You can also use other ready-to-use gel systems such as E-gel TM (Invitrogen) to quickly determine your PCR yield. Read and understand the MSDSs provided by the chemical manufacturer before you store, handle, or work with any chemicals or hazardous materials. Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 13

24 In a positive control or sample, a single fragment ranging from 300 to 500 bp in size should be detected on a gel. Actual fragment size depends on the fungal species. No product should be visible in a negative control reaction. DNA Mass Ladder 2.0kb 1.2kb 0.8kb 0.4kb Positive Control Negative Control Sample X Note: If your samples show no PCR product, PCR inhibition is the most likely cause. Troubleshooting on page 23 provides more information about potential PCR problems and solutions. 0.2kb 0.1kb GR2292 Purifying PCR Products for Cycle Sequencing From the remaining 25 µl of PCR product mixture, remove unused dntps and primers using one of the following products: ExoSAP-IT (USB PN 78200) Read and understand the MSDSs provided by the chemical manufacturer before you store, handle, or work with any chemicals or hazardous materials. Montage PCR Filter Unit (Millipore PN UFC7 PCR50) Be sure you follow the guidelines for the starting sample volume for cleanup as directed in the product literature. 14 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

25 Performing Cycle Sequencing Performing Cycle Sequencing Cycle sequencing occurs when successive rounds of denaturation, annealing, and extension in a 9800 Fast Thermal Cycler result in the incorporation of dye terminators into extension products. The products are then loaded into a genetic analyzer to determine the D2 rdna fungal sequence. Note: You can use a GeneAmp PCR System 9700 (in 9600 emulation mode) instead of a 9800 Fast Thermal Cycler, but the 9700 does not provide the reduced amplification and sequencing times allowed by the new FAST Microseq D2 PCR chemistry and the 9800 Fast Thermal Cycler. For additional information about cycle sequencing chemistries, refer to the Automated DNA Sequencing Chemistry Guide (PN ). Preparing Cycle Sequencing Reactions Prepare one forward and one reverse sequencing reaction for each PCR product. CHEMICAL HAZARD. MicroSeq D2 LSU rdna Fungal Sequencing Mixes (Forward and Reverse) can cause eye, skin, and respiratory tract irritation. Read the MSDS, and follow the handling instructions. Wear appropriate protective eyewear, clothing, and gloves. 1. In a reaction tube or 96-well plate, combine in parallel for each PCR product: 7 µl of the purified PCR product + 13 µl of the forward sequencing mix 7 µl of the purified PCR product + 13 µl of the reverse sequencing mix 2. Cap the tubes or seal the 96-well plate with the 96-well heat seal, then place in the thermal cycler. Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 15

26 Performing Cycle Sequencing 1. Program the 9800 Fast Thermal Cycler or the GeneAmp PCR System 9700 (in 9600 emulation mode) using the following thermal-cycling conditions: Initial Step Each of 25 Cycles Melt Anneal Extend Final Step HOLD CYCLE HOLD 96 C 1 min 96 C 10 sec 50 C 5 sec 60 C 1 min 15 sec 4 C 2. Set the reaction volume for thermal cycling to 20 µl. 3. Start the run. 4. If you are using a CentriSep Spin column to purify extension products (see the section below), hydrate the column. 5. If necessary, store the extension products overnight at 4 C before purifying them. You can store extension products at 20 C for up to 1week. Purifying Extension Products After cycle sequencing, excess dye terminators and primers must be removed from the cycle sequencing reactions using one of the following products. If you performed PCR in... Purify using... MicroAmp tubes DyeEx 2.0 Spin Kit (Qiagen PN 63204) or CentriSep Column (Applied Biosystems PN ) or Performa DTR Gel Filtration Cartridges (Edge Biosystems PN 98780) 16 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

27 Performing Electrophoresis of Extension Products If you performed PCR in... Purify using well plates Performa DTR Ultra 96-Well Plate Kit (Edge Biosystems PN 54789) or DyeEx 96 Kit (Qiagen PN 63181) Follow the guidelines and procedures that come with the kits. Performing Electrophoresis of Extension Products CHEMICAL HAZARD. Formamide. Exposure causes eye, skin, and respiratory tract irritation. It is a possible developmental and birth defect hazard. Read the MSDS, and follow the handling instructions. Wear appropriate protective eyewear, clothing, and gloves. Configuring the Instrument for Electrophoresis First, configure your data collection software as described in the MicroSeq ID Analysis Software Version 2.0 Getting Started Guide, Appendix A, Using Autoanalysis with Applied Biosystems 3130/3130xl Genetic Analyzers. Use only the 50-cm capillary array length regardless of the instrument that you are using. Refer to your instrument user guide for more information. Then select the Run Module, Basecaller, and Dye/Set Primer specified in the following table. Instrument Filter Set Run Module Basecaller DyeSet/Primer (Mobility File) Applied Biosystems 3130 or Applied Biosystems 3130xl E StdSeq50_POP6_1 KB.bcp KB_3130_POP6_BDT v1.mob file Note: You can use POP7 polymer with the StdSeq50_POP7 run module and the KB_3130_POP7_BDT v1.mob file. However this instrument configuration reduces data quality within the first 40 bases on the 5' end of the sequence. Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 17

28 Refer to the MicroSeq ID Analysis Software Online Help for more information about naming conventions for Basecaller and DyeSet/Primer files. Performing the Run 1. Dispense 27 µl of Hi-Di TM formamide into each well of a 96-well plate (PN ), to which you will add purified cycle-sequencing reaction products. 2. Add 3 µl of purified extension product to each well. Note: Dilution in Hi-Di TM formamide normalizes the signal strength of the sequencing reaction and stabilizes extension products. If after a 1:10 dilution you do not detect a sequencing ladder due to a low signal, dilute the purified extenstion product 1:1 in Hi-Di TM formamide before the run, or rerun the sample without diluting. Samples producing a very high signal can be diluted 1:40 or higher, before the run. 3. Mix by pipetting up and down. 4. Spin the plate to remove bubbles from the bottom of the wells. 5. Store the rest of the purified extension product at 20 C. 6. Load the plate into your instrument. 7. Start the run. 8. When the run is complete, analyze the data using the MicroSeq ID Analysis Software. Note: For information on using the software, refer to the MicroSeq ID Analysis Software Online Help, the MicroSeq ID Analysis Software Version 2.0 Quick Reference Card, and the MicroSeq ID Analysis Software Version 2.0 Getting Started Guide. 18 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

29 Analyzing Data Analyzing Data MicroSeq ID Analysis Software MicroSeq Proprietary Libraries MicroSeq ID Analysis Software analyzes sequences obtained with any of the MicroSeq Microbial Identification Kits. The software assembles the D2 region sequence for the unknown, then compares the sequence with D2 region sequences in the MicroSeq ID Fungal Gene Library. Based on the comparison, the software provides a potential ID for the unknown fungal species. With the software, you can perform: Basecalling with assignment of quality values Clear-range determination, which lets you exclude data near sequence ends (typically poor-quality data) from analysis Assembly and alignment of sequences to generate a high-quality consensus sequence Comparison of the consensus sequence to the MicroSeq ID proprietary libraries to generate a list of the closest matches, including percentage match scores Exports of projects and consensus sequences to facilitate datasharing between collaborators The software also has features that assist with 21 CFR Part 11 compliance requirements. For more information, refer to the MicroSeq ID Analysis Software Version 2.0 Quick Reference Card and the MicroSeq ID Analysis Software Version 2.0 Getting Started Guide provided with the software. The MicroSeq ID Fungal Gene Library includes over 1,100 validated D2 rdna fungal sequences. All sequences and strains are carefully checked and quality controlled to ensure maximum reliability. Polymorphic positions are taken into account to ensure the highest degree of accuracy. Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 19

30 Custom Libraries MicroSeq Reports In addition to accessing the proprietary libraries, MicroSeq ID Analysis Software allows you to create custom libraries. You can create custom libraries using data generated by the MicroSeq ID software, or using downloaded sequences from public databases. Custom libraries are easy to import and export, making information sharing convenient. During the analysis process, you can search proprietary and custom libraries simultaneously to determine the 20 closest matches to the sequence of your unknown fungal species. MicroSeq ID Analysis Software generates four detailed reports: Analysis QC Report Allows you to quickly scan the unknowns in a project to gather information about the samples, including the top percent identity match and specimen score to measure data quality. Figure 1 on page 21 shows an example Analysis QC Report. Library Search Report Provides more detailed information about the libraries that were searched, including a list of all the top matches and the total number of bases searched. Figure 2 on page 22 shows an example Library Search Report. Audit Trail Report Tracks changes made to projects after analysis. Electronic Signature History Report Provides a summary of the electronic signatures used in a project. All reports can be generated on a project level and on a per specimen level. In addition, the software allows you to create custom reports. For information, refer to the MicroSeq ID Analysis Software Version 2.0 Online Help. 20 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

31 Analyzing Data Figure 1 Example Analysis QC Report Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 21

32 Figure 2 Example Library Search Report 22 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

33 Troubleshooting Troubleshooting Problem Possible Cause Solution No PCR product PCR inhibition Make additional dilutions (1:10, 1:100, 1:1000) of the working stock (see page 10) before proceeding to PCR. Short sequence, the first part of which is very bright and off-scale and the remainder of which has very low intensity Both results and raw data show occasional high spikes for all four dye colors. Large regions of overlapping sequence or Cannot call bases for large regions of sequence Bacterial sample Cells were not disrupted by the PrepMan Ultra method. High starting amount of DNA or too much DNA template in the sequencing reaction Bubbles in the capillary DNA sample is contaminated (that is, the DNA is derived from more than one species of fungi). Use the MicroSeq 500 or the MicroSeq Full Gene 16S rdna Bacterial Identification Kit. Use the bead-beating method to isolate fungal genomic DNA or bacterial genomic DNA ( Decrease the amount of fungal cell material (smaller colony or pellet). or Estimate PCR product yield on agarose gel and use 5 to 20 ng of amplicon for sequencing as described on page 13. Check the instrument manual. Check for pipetting errors, sub-culture the organism. or Clone the PCR product (using a kit such as the Invitrogen Topo PCR Cloning Kit) before performing sequencing. Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 23

34 Problem Possible Cause Solution Small regions of overlapping sequence In fungal species with multiple copies of the rrna gene: Insertions or deletions in a subset of the genes can result in a shift by 1 to 3 bp. The gene can be polymorphic, resulting in overlap of up to 1% of the sequence. No action needed. 24 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

35 Frequently Asked Questions Frequently Asked Questions Running 30 Cycles Instead of 35 Cycles Sensitivity and Quantification If you are running fungal and bacterial samples on the same plate, you can run the fungal samples for 30 PCR cycles (the recommended number of cycles for bacterial samples). However, you may see some fungal drop-out at 30 cycles. Using the 9800 in STD mode or the 9700 in MAX mode may significantly decrease the drop-out rate at 30 cycles. What is the sensitivity of the MicroSeq Fungal Identification Kit? As long as you start from a visible colony or cell pellet, MicroSeq kits will work. Can I use the MicroSeq Fungal Identification Kit to quantify fungi or yeast? No. The PCR is an endpoint assay. Sample Preparation and Storage What is the best way to prepare yeast samples? Prepare yeast samples using the PrepMan Ultra Sample Preparation Reagent or bead-beating method, just as you prepare bacterial samples. Extra dilutions of the working fungal stock are sometimes necessary. Which kit should I use to identify yeast samples? Use the MicroSeq Fungal Identification Kit to sequence and identify yeast samples. Are there alternative methods for preparing genomic DNA? If the PrepMan Ultra kit method does not successfully disrupt cells, you can use the bead-beating method to isolate genomic DNA. Use 100 µm zirconia/silica beads (Biospec Products PN Z). Refer to for the bead-beating protocol. Alternatively, you can use a DNA extraction kit (available from various vendors) to isolate pure DNA. Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 25

36 Can I use less PrepMan Ultra Sample Preparation Reagent if I start with a smaller colony? Yes. The ideal colony size is 2 to 3 mm. For smaller colonies, you can decrease the amount of PrepMan Ultra Sample Preparation Reagent to 50 µl from the suggested 100 µl in the PrepMan Ultra Sample Preparation Reagent Protocol (PN ). Can I enrich my genomic DNA by using less PrepMan Ultra Sample Preparation Reagent? Yes. However, be careful not to overload the PCR mix. Enriched samples tend to have more cellular and other debris, which can interfere with PCR. At what temperature should I store my PrepMan Ultra-isolated DNA? Applied Biosystems recommends storing DNA at 20 C, although you may safely keep it at room temperature or 4 C overnight. Contamination How can I tell if my sequence is representative of a single species? The DNA sequence from a single species should be distinct (easy to call base pairs), without significant regions of overlapping sequence. If my initial DNA sample is contaminated (that is, it comes from multiple species), how can I sequence my PCR product? Clone the PCR product using a kit such as the Topo PCR Cloning Kit from Invitrogen. Overlapping Sequences My sequence has large regions of overlap (>5% mixed bases). What does this mean? The presence of large regions of overlapping sequence indicates that the DNA is derived from more than one species of fungi or bacteria. To resolve this presence: Sub-culture the organism to pure culture and repeat identification. or Clone the PCR product (using a kit such as the Invitrogen Topo PCR Cloning Kit) before sequencing. 26 Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol

37 Frequently Asked Questions My sequence has small regions (up to 1%) of overlap. What does this mean? No action is needed. Some fungal and bacterial species can have multiple copies of the rrna gene. Small regions of overlapping sequence can be caused by insertions or deletions in a subset of these genes, resulting in a shift of 1 to 3 bp. Similarly, the gene can be polymorphic, leading to overlap of up to 1% of the sequence. PCR Product Size Can I always expect the same size PCR product for all species? PCR products can vary from the expected product size, depending on the species. Expected product sizes for the: MicroSeq Fungal Kit 1 band at 300 to 500 bp MicroSeq 500 Kit 1 band at 460 to 560 bp MicroSeq Full Gene Kit 1 band at 460 to 560 bp and 2 bands at 700 to 800 bp Can I increase the number of cycles to increase the PCR yield? Yes, but doing so can cause additional background signal from the negative control. Species Libraries How are species in the Applied Biosystems libraries validated? Refer to the MicroSeq kit Validation Statement link at Where are the species in the Applied Biosystems libraries derived from? The species are derived from the American Type Culture Collection (ATCC) and the Deutsche Sammlung von Mikroorganismen und Zellkulturen GmbH (German Collection of Microorganisms and Cell Cultures). Are there pathogenic species included in the libraries? Yes, but pathogenicity of the isolates needs to be further confirmed by additional testing, such as in the case of E.coli O157:H7. Fast MicroSeq D2 LSU rdna Fungal Identification Kit Protocol 27

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