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Maize Dwarf Mosaic Virus(MDMV)玉米矮小花叶病毒RT-PCR试剂盒上海圻明生物优势供应。更多产品资料欢迎免费咨询。
One of the many important uses of PCR technology is that it can be used to label DNA probes with high specific activity. PCR technology has high specificity, and can synthesize probe DNA fragments in quantities within 1~2h if [α-32P]dNTP or other markers are added to the substrate
dNTPs, the probe DNA can be well labeled during DNA synthesis, and the incorporation rate of the marker can be as high as 70%~80%. Therefore, PCR labeling technology is particularly suitable for large-scale detection and non-radiolabeling. The disadvantage of this method is that a specific pair of PCR primers is synthesized.
Labeling can also be achieved by using small fragments prepared from probe DNA as primers.
Solution preparation
1. Prepare a stock solution
Unless otherwise stated, all unused stock solutions should be divided into disposable aliquots and stored at -20 °C after preparation. Avoid repeated freeze-thaw cycles.
1.1* Acid Stock Solution (125X):
Add 20 μL DMSO to *ate (component B) to make a 125X* acid stock solution.
2. Prepare standard solutions
*Salt standard solution
Add 50 μL of 1 mM KH2PO4 (Component C) to 950 μL of deionized water or enzyme reaction buffer to give a 50 μM * saline standard solution (PS7). A 50 μM * saline standard solution (PS7) was taken and serially diluted 1:2 to obtain a serially diluted phosphate standard with deionized water or enzyme reaction buffer.
3. Prepare a working solution
Add 20 μL of 125X* stock solution to 2.5 mL of sterile H2O and mix well to make a working solution of *salt. Avoid potential Pi contamination. Note: Avoid direct exposure of *salts (component B) to light. Due to the high sensitivity of this assay to Pi, it is extremely important to use Pi-free labware and reagents.
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文献和实验on the brome mosaic virus (BMV) which allows gene silencing in different cereals including barley (Hordeum vulgare ), wheat (Triticum aestivum ), and maize (Zea mays ). Infection of maize plants by the corn smut fungus Ustilago maydis leads
MCMV 和 SCMV 复合侵染玉米引起玉米组织中 siRNAs 的积累
后的病毒 RNA 可以被 RDR 识别,并将其加工成双链 RNA,再一次被 DCL 蛋白切割形成次级 vsiRNA.初级和次级 vsiRNA 没有本质上的区别,都可以作用于靶标,发挥抗病毒的功能。 玉米褪绿斑驳病毒(MCMV)与侵染玉米的马铃薯 Y 病毒科病毒,如玉米矮花叶病毒(MDMV)、小麦条纹花叶病毒(WSMV)和甘蔗花叶病毒(SCMV),复合侵染时引起玉米致死性坏死(MLN),对玉米产量造成很大的威胁。虽然有报道称马铃薯 Y 病毒属病毒编码的沉默抑制子 HC-Pro 可以增加异源病毒
MCMV 和 SCMV 复合侵染玉米引起玉米组织中 siRNAs 的积累
的靶标,被切割后的病毒 RNA 可以被 RDR 识别,并将其加工成双链 RNA,再一次被 DCL 蛋白切割形成次级 vsiRNA.初级和次级 vsiRNA 没有本质上的区别,都可以作用于靶标,发挥抗病毒的功能。 玉米褪绿斑驳病毒(MCMV)与侵染玉米的马铃薯 Y 病毒科病毒,如玉米矮花叶病毒(MDMV)、小麦条纹花叶病毒(WSMV)和甘蔗花叶病毒(SCMV),复合侵染时引起玉米致死性坏死(MLN),对玉米产量造成很大的威胁。虽然有报道称马铃薯 Y 病毒属病毒编码的沉默抑制子 HC-Pro
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