Wheat aphid and multiplex PCR (polymerase chain reaction) detection kit of parasitic wasp thereof
A kit and aphid technology, applied in the field of multiplex PCR detection, can solve the problems of time-consuming and laborious, difficult to identify species, etc.
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Embodiment 1
[0091] Example 1 The specific amplification effect of multiplex PCR system MP1 on target species
[0092] 1. Genome preparation of target aphid species
[0093] The single-headed barley aphid, barley barley, barley aphid, and barley aphid were placed in 1.5 mL centrifuge tubes for tissue grinding and DNA extraction. The centrifuge tubes for storing different aphid DNA solutions were marked on the label. Species name, reserve at -20°C.
[0094] 2. To synthesize the primers required in the multiplex PCR system MP1, see the four pairs of primers corresponding to the MP1 system in Table 1. Each pair of primers was prepared into a mixed primer solution in proportion, and the final concentration of each primer in the reaction system was shown in Table 1.
[0095] 3. The PCR amplification reaction system is calculated in 10 μL, including ddH 2 O, 2.0 μL; 2×Multiplex PCR MasterMix, 5.0 μL; Primer Mix, 1.0 μL; 10 μg / μL BSA, 0.5 μL and DNA template, 1.5 μL.
[0096] The PCR reaction...
Embodiment 2
[0099] Example 2 Multiplex PCR System MP2 Specific Amplification Effect on Target Species
[0100] 1. Preparation of the genome of the target parasitoid species
[0101] The single-headed winged aphids, Aphididae, Uzbekia, Aphidia, and Aphidia were placed in 1.5mL centrifuge tubes for tissue grinding and DNA extraction, and the centrifuge tubes storing DNA solutions of different parasitoids were marked with Species name, spare at -20°C.
[0102] 2. For the primers required in the synthesis of the multiplex PCR system MP2, see the corresponding primers for the MP2 system in Table 1. Each pair of primers was prepared in proportion to a mixed primer solution, and the final concentration of each primer in the reaction system is shown in Table 1.
[0103] 3. PCR amplification reaction system is calculated in 10 μL, including ddH 2 O, 1.8 μL; 2×Multiplex PCR Master Mix, 5.0 μL; Primer Mix, 1.0 μL; 10 μg / μL BSA, 0.5 μL; 5M TMAC, 0.2 μL and DNA template, 1.5 μL.
[0104] The PCR r...
Embodiment 3
[0107] Example 3 Multiplex PCR System MP3 Specific Amplification Effect on Target Species
[0108] 1. Preparation of the genome of the target parasitoid species
[0109] Refer to Example 2 for the extraction methods of Chrysopus spp., Aphids aphids Phaenoglyphis villosa and Phaenoglyphis villosa.
[0110] 2. Synthesize the primers required in the multiplex PCR system MP3. The primer sequences in the system and the final concentration of each primer in the reaction system are shown in Table 1.
[0111] 3. PCR amplification reaction system is calculated in 10 μL, including ddH 2 O, 2.0 μL; 2×Multiplex PCR MasterMix, 5.0 μL; Primer Mix, 1.0 μL; 10 μg / μL BSA, 0.5 μL and DNA template, 1.5 μL.
[0112] The PCR reaction conditions were: pre-denaturation at 95°C for 15 minutes; denaturation at 94°C for 30 seconds, annealing at 58°C for 1 minute and 30 seconds, and extension at 72°C for 1 minute, a total of 35 cycles.
[0113] 4. Identification of PCR products Take 5.0 μL of PCR amp...
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