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How Do We See Our DNA?

How Do We See Our DNA?. Horizontal Agarose Gel Electrophoresis. Pour gel Sample preparation depends on Application Electrophoresis (constant voltage) detect with fluorescent dye (eg., ethidium bromide, SYBR, etc). Equipment. Loading the Gel. How It Works.

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How Do We See Our DNA?

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  1. How Do We See Our DNA?

  2. Horizontal AgaroseGel Electrophoresis • Pour gel • Sample preparation depends on Application • Electrophoresis (constant voltage) detect with fluorescent dye (eg., ethidium bromide, SYBR, etc)

  3. Equipment

  4. Loading the Gel

  5. How It Works • The DNA samples are loaded into wells of an agarose gel and electrophoresed, along with loading dyes. • An electrical field applied across the gel causes the DNA fragments in the samples to move from their origin (a sample well) through the gel matrix toward the positive electrode. Why? • Small DNA fragments migrate faster than larger ones. •   The loading dyes are of 2 different sizes, corresponding to very small DNA fragments and very large DNA fragments. 

  6. The PV92 Alu insertion is inherited in a simple Mendelian pattern with each parent contributing one "Allele" to the offspring. If an allele for the PV92 Alu insertion is represented by (+) and the absence of the allele is indicated by (-), the three possible genotypes can be expressed as (+/+), (+/-) and (-/-). Their inheritance can be summarized as follows: • (-/-)neither parent contributed Alu insertion • (+/-)received Alu insertion from one parent • (+/+)both parents contributed Alu insertion

  7. ALU Gel Example Human DNA typing by the Molecular Biology Lab:  Determination of an ALU insertion polymorphism by PCR

  8. Take A Picture!!!

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