Servicebio 水平電泳槽(含藍光光源) SVL-2

ProductOverview

SVL-2 integrated horizontal electrophoresis instrument is mainly used for rapid agarose electrophoresis separation experiments of small amounts of DNA and RNA samples.

Product Features

1. The gel maker mold is integrally formed, which can make four different sizes ofgel blocks.

2. Standard blue light transilluminator, with SPW-6S electrophoresis power supply, can directly observe the band during the electrophoresis process.

3. The transparent upper cover has a hole design, which is convenient for heat dissipation and observation.

4. Card slot limit function, accurate operation.

5. The electrode holder and electrode head are detachable, which is convenient for cleaning and maintenance.

Product structure

Product Specifications

OperationSteps

Please ensure that the horizontal electrophoresis tank, gel tray, sample comb, gel maker and other components are clean and dry before gel preparation.

1. Preparation

Weigh an appropriate amount of agarose into an Erlenmeyer flask, add an appropriate amount of buffer, place it in a water bath, a magnetic heating stirrer or a microwave

2.Gel Making

Place the gel maker horizontally on the experimental bench, select a suitable gel tray (different sizes of gel trays are selected according to different experimental needs, the specifications of the gel tray are 120mmXmmperimental needs, the specifications of the gel tray are 120mmXmmmmm X60mm), put the gel tray Place it in thegel maker (two pieces of 60mmX60mm gel can be made at the same time, and only one piece can be made for other specifications) and put the sample comb in a fixed position. Add 5ul SerRed (or other nucleic acid dyes) solution to the agarose gel cooled°C 50°C . After mixing, carefully pour it into the gel tray, and slowly spread the gel until the entire surface of the gel tray is uniform. For thegel layer, let stand at room temperature until the gel is completely solidified, and then gently pull out the sample comb vertically to complete the preparation of thegel plate.

3.Sample Loading

Take the prepared gel and the gel tray out of the gel maker together and place them in the electrophoresis box with the sample addition hole close to the negative electrode (black is the negative electrode)。

Use a 10ul micropipette to add the samples to the sample grooves of the rubber plate respectively. After each sample is added, a sample addition head should be replaced to prevent contamination. When adding sounds pay attention to the order of adding samples) .

4.  Electrophoresis

Cover the top cover according to the correct position of the positive and negative poles (red is positive, black is negative), insert the electrophoresis wire into the electrophoresis power supply according to the correct color, pprise 片面specific electrophoresis parameters are adjusted according to the actual experimental parameters) .

The sample moves from the negative (black) to the positive (red) direction. As the voltage increases, the effective separation range of the agarose gel decreases. The electrophoresis was stopped when the bromophenol blue ved to about blue of the about blue 10enol blue ved to about blue ？ the gel plate.

5.  Obsersation

Thisintegrated horizontal electrophoresis instrument is equipped with a blue lightlight transilluminator, which can observe the electrophoresis situation in real time with ( SPW-6S electrophoresis power supply ).

Product configuration list

Precautions

1. Do not operate this product with electricity (the top cover of the horizontal electrophoresis apparatus must be covered before the electrophoresis power is turned on after the sample is added, and do not is turned on after the sample is added, and do notled, and do not theduel the hemis sioned, and do notimel the huslly oid the danger of electric shock).

2. All parts of this product can be washed with water, just dry naturally or dry with absorbent paper. Do not bake at high temperature to avoid damage to the product.