Plant Methods | |
Protocol: a fast and simple in situ PCR method for localising gene expression in plant tissue | |
Matthew Gilliham1  Simon J Conn2  Rachel A Burton5  Weng W Ng1  Gwenda M Mayo3  Charlotte Jordans1  Vanessa M Conn1  Sandra K Tanz4  Asmini Athman1  | |
[1] Waite Research Institute & School of Agriculture, Food and Wine, University of Adelaide, PMB1, Glen Osmond, SA 5064, Australia;Centre for Cancer Biology, Division Immunology, Level 3, Frome Road, Adelaide, SA, Australia;Adelaide Microscopy Waite Facility, University of Adelaide, Glen Osmond, SA, Australia;ARC Centre of Excellence in Plant Energy Biology, The University of Western Australia, Perth, WA, Australia;ARC Centre of Excellence in Plant Cell Walls, University of Adelaide, Glen Osmond, SA, Australia | |
关键词: Immunohistochemistry; Plant tissue; Cell-specific localisation; RT-PCR; In situ PCR; | |
Others : 1151524 DOI : 10.1186/1746-4811-10-29 |
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received in 2014-05-23, accepted in 2014-09-10, 发布年份 2014 | |
【 摘 要 】
Background
An important step in characterising the function of a gene is identifying the cells in which it is expressed. Traditional methods to determine this include in situ hybridisation, gene promoter-reporter fusions or cell isolation/purification techniques followed by quantitative PCR. These methods, although frequently used, can have limitations including their time-consuming nature, limited specificity, reliance upon well-annotated promoters, high cost, and the need for specialized equipment. In situ PCR is a relatively simple and rapid method that involves the amplification of specific mRNA directly within plant tissue whilst incorporating labelled nucleotides that are subsequently detected by immunohistochemistry. Another notable advantage of this technique is that it can be used on plants that are not easily genetically transformed.
Results
An optimised workflow for in-tube and on-slide in situ PCR is presented that has been evaluated using multiple plant species and tissue types. The protocol includes optimised methods for: (i) fixing, embedding, and sectioning of plant tissue; (ii) DNase treatment; (iii) in situ RT-PCR with the incorporation of DIG-labelled nucleotides; (iv) signal detection using colourimetric alkaline phosphatase substrates; and (v) mounting and microscopy. We also provide advice on troubleshooting and the limitations of using fluorescence as an alternative detection method. Using our protocol, reliable results can be obtained within two days from harvesting plant material. This method requires limited specialized equipment and can be adopted by any laboratory with a vibratome (vibrating blade microtome), a standard thermocycler, and a microscope. We show that the technique can be used to localise gene expression with cell-specific resolution.
Conclusions
The in situ PCR method presented here is highly sensitive and specific. It reliably identifies the cellular expression pattern of even highly homologous and low abundance transcripts within target tissues, and can be completed within two days of harvesting tissue. As such, it has considerable advantages over other methods, especially in terms of time and cost. We recommend its adoption as the standard laboratory technique of choice for demonstrating the cellular expression pattern of a gene of interest.
【 授权许可】
2014 Athman et al.; licensee BioMed Central Ltd.
【 预 览 】
Files | Size | Format | View |
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20150406083627542.pdf | 2994KB | download | |
Figure 4. | 156KB | Image | download |
Figure 3. | 111KB | Image | download |
Figure 2. | 339KB | Image | download |
Figure 1. | 93KB | Image | download |
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