Dilutions & Separation Techniques Flashcards

1
Q

What formula is used to make a fixed amount of a dilute solution from a stock solution?

A

C1V1 = C2V2

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2
Q

What is V1?

A

The volume of stock solution needed to make the new solution.

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3
Q

What is V2?

A

The final volume of the new solution.

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4
Q

What is C1?

A

The concentration of stock solution.

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5
Q

What will a buffer do?

A

Control pH especially in proteins.

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6
Q

What does a colorimeter measure?

A

How much a solution will absorb in a particular wavelength.

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7
Q

What separation techniques are used by biologists?

A
  • Filtration
  • Fractional distillation
  • Paper/thin layer chromatography
  • Centrifugation
  • Iso-electric point
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8
Q

What does filtration separate?

A

A solid from a liquid.

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9
Q

What does distillation use to separate substances?

A

Boiling point.

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10
Q

What does centrifugation use to separate substances?

A

Molecular weight.

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11
Q

What is the iso-electric point?

A

The pH at which a protein has no net charge.

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12
Q

What can be used as the defining value for proteins?

A

the iso-electric point.

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13
Q

How can IEP be calculated?

A

By using info on all of the amino acid/basic characteristics and their number in the protein.
It can also be measured using a gel set up with a pH gradient and measuring the pH the protein migrates to.

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14
Q

What is a linear dilution?

A

One where the dilutions differ by an equal interval.

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15
Q

What is a log dilution?

A

One in which the dilutions differ by a constant proportion.

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16
Q

How does a pH buffer allow the pH of a reaction mixture to be kept constant?

A

As the addition of acid or alkali have a very small effect on the buffer.

17
Q

What is affinity chromatography used for?

A

To separate proteins.

18
Q

How is affinity chromatography carried out?

A

A solid matrix of gel column is created with specific molecules bound to the matrix or gel. Soluble, target proteins in a mixture with a high affinity for these molecules become attached to them as the ,mixture passes down the column. Other non-target molecules with a weaker affinity are washed out.