BIOL 3120 Cell Biology Lab - Lab 6 PDF

Summary

This document outlines the procedures for genomic DNA and total RNA extraction, along with the objectives and precautions for working with RNA. It details the principles behind DNA and RNA extraction. Lab instructions and a discussion about the lab are also included.

Full Transcript

BIOL 3120 - Cell
Biology Lab
Lab 6. Genomic DNA extraction; &
Total RNA Extraction (Demo)

Rubaia Tasmin
10/14/2024

Email: [email protected]

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Today’s Lab Objectives

1. Understand the principles of genomic DNA extraction from plant
tissue

2. Extract genomic DNA from plant tissue (Arabidopsis thaliana
leaf sample)

3. Measure the concentration and assess the purity of the genomic
DNA extracts

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Principal of DNA extraction
in plants

Add isopropanol to
precipitate and 70% ethanol
Disrupt the cell wall Separate DNA to wash the DNA
and plasma from organic
phase Add water to solubilize the
membrane
DNA. The polar water
molecules surrounds the
charged regions of DNA,
allowing it to dissolve. 3
Extraction Buffer
1.50 mM Tris-HCl: maintain the pH at the optimal condition for
DNA extraction
2.10 mM EDTA : EDTA binds to metal ions, like magnesium and
calcium, which are cofactors of DNase; thus preventing the
degradation of DNA.
3.100mM NaCl: dissolves the DNA and maintains its stability
4.1.0 % SDS: SDS causes protein denaturation and disrupts the
interactions between proteins and lipids in cell membranes,
causing the cell to break down and release its contents.
5.10mM β-mercaptoethanol: a strong reducing agent that breaks
the disulfide bonds of proteins, making them insoluble in water to
obtain pure DNA that is free from protein contamination.
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Potassium acetate and Isopropanol
/ethanol
Potassium acetate (Bio 101 Solution III)
Creates a high-salt environment, and neutralizes the
high pH of the lysis solution, facilitating the
precipitation of SDS-bound proteins and other
cellular debris.
Isopropanol / ethanol
The isopropanol facilitates the interaction of K+ or
Na+ with the PO3− groups on the sugar phosphate
backbone of nucleic acids. This interaction makes
the DNA molecule less soluble in water, precipitating
the DNA.

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DNA qualification and
quantification
1. The concentration and purity can be
measured by NanoDrop
spectrophotometer.

2. Nucleic acids and proteins have an
absorbance maxima at 260nm and 280nm,
respectively. Pure DNA will have an
A260/A280 ratio of 1.8–2.0.

3. Lower 260/280 ratios usually indicate
that a sample is contaminated by residual
phenol, sugar, or the reagents used in the 6
 Lab 6 Report Requirements
1. Introduction: Principal of Genomic DNA extraction and purpose of the lab.
2. Materials: All the chemicals, along with concentration, and instruments
used.
3. Methods: Brief steps for the experiment you did.
4. Results:
The concentration of your extracted genomic DNA
The 260/280 ratio of the genomic DNA
Keep the DNA in the freezer for next lab
5. Discussion/conclusion: Interpret your results. Discuss unexpected
findings. What improvements can you make? What is your conclusion? What is
the significance of the lab?
6.
FileLab manual
name for yourquestions & underlined questions
lab report submission-
BIOL3120_Section_Lastname_Firstname_
None
Lab 6​

Send me the Word document by email
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 BIOL 3120 - Cell
Biology Lab

Total RNA Extraction (Demo)

Zijie Zhang
10/08/2024

Email: [email protected]

8
Today’s Lab Objectives
(cont.)

1. To learn the precautions for working with RNA.

2. To learn the principle of RNA extraction

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Precautions for working
with RNA
 Keep the RNA samples intact by placing on ice while in
use

- For long term storage: store RNA samples in –80°C
 Control the source of RNase

- Use RNase-free pipette tips and microcentrifuge tubes
 Clean work area and pipettes with RNaseAway

 Wear clean gloves, masks and lab coat

 Inactivate the RNase using DEPC water
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Principle of RNA extraction in
plants

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RNA assessment

https://www.promega.com/resources/pubhub/methods-of-rna-quality-
assessment/
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