- Компоненты набора реагентов
| Технические характеристики | 50Т | 100Т |
| Кот. Нет. | SN0305AD | SN0306AD |
| RNA Extraction Columns (набор) | 50 (набор) | 100 (набор) |
| DNA Clean-Up Columns (набор) | 50 (набор) | 100 (набор) |
| RNA Extraction Buffer I | 30 мл | 2×30 мл |
| Inhibitor Removal Buffer | 30 мл | 2×30 мл |
| Промывной буфер 1 | 15 мл | 2×15 мл |
| Элюирующий буфер | 20 мл | 20 мл |
| Инструкция по эксплуатации | 1 | 1 |
- Хранилище
This reagent kit can be stored at room temperature (15-25℃) in a dry environment and is stable for 12 месяцы.
- Инструкции по использованию набора реагентов
3.1 This kit is intended for molecular biology research purposes and should not be used for disease diagnosis or treatment.
3.2 Some components in the kit contain irritants; it is advisable to take necessary precautions (such as wearing protective clothing and goggles).
3.3 The use of this kit requires additional equipment such as a high-speed centrifuge, водяная баня (металлическая ванна), вихревой смеситель, безводный этанол, liquid nitrogen, chloroform, стерильная деионизированная вода, and EP tubes.
- Знакомство с набором реагентов
This RNA purification kit provides a fast and efficient method for purifying polysaccharide and polyphenol plant total RNA, suitable for most polysaccharide and polyphenol-rich plant tissues. In general, plant tissues rich in polysaccharides and polyphenols contain a high level of secondary phenolic metabolites and polysaccharides, significantly affecting RNA extraction efficiency. This kit can effectively remove polysaccharides and polyphenols, as well as efficiently eliminate DNA contamination from samples. If the experiment is sensitive to DNA, it is recommended to use primers spanning introns for downstream experiments.
The RNA Fast Purification Kit can extract total RNA from plant tissues (including nuclear RNA and cytoplasmic RNA) в пределах 1 час. The extracted RNA can be directly used for RT-ПЦР, Нозерн-блоттинг, и т. д.. Весь процесс очистки не требует использования токсичных реагентов типа фенол-хлороформа., making this RNA purification kit suitable for various other sample types.
- Экспериментальные принципы и процедуры
- Процесс экстракции
Precautions before starting the experiment:
А. Before using Промывной буфер 1, add the specified amount of absolute ethanol according to the label on the reagent bottle, and check the box on the label to indicate that absolute ethanol has been added.
Б. The Elution Buffer is a 0.1х ТЕ решение containing minimal EDTA. If EDTA affects subsequent experiments, it is recommended to replace the Elution Buffer with sterile deionized water.
- Образец обработки:
А. Material Collection and Storage:
If fresh materials cannot be used immediately, place them in liquid nitrogen and store them at -80°C.
Б. Whenever possible, collect fresh materials, as they contain fewer polysaccharides and polyphenols.
2. Grind approximately 100 mg of fresh samples or not more than 20 mg of dry material using liquid nitrogen.
3. Добавлять 600μl RNA Extraction Buffer I, ensuring there are no blocky tissues in the ground sample. Blocky tissues are difficult to lyse and can reduce RNA yield.
4. Vortex for 30 секунды.
5. Centrifuge the lysate for 5 minutes at 12,000 об/мин.
(Примечание: Polysaccharide plant materials may produce a lot of sticky substances at this step, which can shear RNA in subsequent steps. Поэтому, remove these substances during this step.)
- Transfer the supernatant obtained in the previous step to a DNA Clear Purification Column, центрифуга в 12,000 об/мин для 30 секунды, and collect the filtrate (Примечание: RNA is present in the filtrate).
- Добавлять 250μl of absolute ethanol, mix by pipetting. If there is a small amount of precipitation, it does not affect subsequent experiments. Add the liquid to the RNA purification column, центрифуга в 12,000 об/мин для 30 секунды, and discard the flow-through.
- Добавлять 700мкл буфера для удаления ингибитора to the RNA purification column, центрифуга в 12,000 об/мин для 30 секунды, and discard the flow-through.
- Добавлять 700мкл промывочного буфера 1 to the RNA purification column, центрифуга в 12,000 об/мин для 30 секунды, and discard the flow-through.
- Добавлять 500мкл промывочного буфера 1 to the RNA purification column, центрифуга в 12,000 об/мин для 3 минуты, and discard the flow-through.
- Place the RNA purification column into a new 1.5ml centrifuge tube, air-dry the membrane at room temperature for 2 минуты.
(Примечание: Confirm the addition of ethanol to Wash Buffer 1. The presence of ethanol significantly affects subsequent experiments. Поэтому, membrane drying is crucial. После центрифугирования, ensure the absence of ethanol before elution. Discard the waste and the collection tube. After using Wash Buffer 1, the membrane on the RNA purification column should only have a slight color. Carefully remove the RNA purification column after centrifugation, ensuring it does not touch the collection tube to avoid ethanol contamination.)
- Капать 50-100мкл элюирующего буфера на мембрану, центрифуга в 12,000 об/мин для 1 минута, and collect the RNA solution.
(Примечание: Eluting RNA with 50μl Elution Buffer can increase RNA concentration but decrease total RNA yield.)
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