Northern blotting

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NORTHERN BLOTTING IQRA JABBAR M.PHIL. SCHOOL OF BIOLOGICAL SCIENCES

description

An overview of northern blotting.. with its applications, and pros and cons

Transcript of Northern blotting

Page 1: Northern blotting

NORTHERN BLOTTING

IQRA JABBAR

M.PHIL.

SCHOOL OF BIOLOGICAL SCIENCES

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WHAT IS BLOTTING?

Proteins, DNA or RNA, can be transferred onto a carrier

nitrocellulose or nylon membrane

The transfer of biological samples from a gel to a membrane and their subsequent detection on

the surface of the membrane

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Blotting Types

Southern(DNA)

Northern(RNA)

Western (Protein)

TYPES OF BLOTTING

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NORTHERN BLOTTING

A technique to detect and measure specific

RNA sequences

Developed by James Alwine and George Stark

at Stanford University in 1977

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Oligo (dT) column chromatography can be done to isolate only polyA+ RNAs

Formaldehyde used as denaturing agent in gels to remove secondary structures.

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Nylon membranes are preferred • positively charged• high capacity to bind

nucleic acids• greater robustness on

handling)

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cDNA, RNA, or oligonucleotides with a minimum of 25 complementary bases to the target sequence.

Probes can be Radioactive (Radiolabelled with P32) Or Chemiluminiscent (probe attached to enzyme for chemiluminiscent substrate or to a ligand..)

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Steps involved in northern blotting

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BLOTTING SET UP

Transfer buffer contains formamdie• It lowers the annealing temperature for probe-

RNA • Prevents RNA degradation at high

temperatures.

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CHEMILUMINISCENT PROBES

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APPLICATIONS OF NORTHERN BLOTTING

To observe a particular gene’s expression

pattern between

Tissues Organs Developmen

tal stages

Environmental stresses

Pathogen infection

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APPLICATIONS OF NORTHERN BLOTTING

Comparison of

expression of

oncogenes and tumor

suppressor

genes between

cancerous and normal

tissues

Normal Cancerous

Oncogene

Tumor suppressor

gene

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APPLICATIONS OF NORTHERN BLOTTING

By using only one probe.. If obtain

variance in the level of each

band….

• May be alternative spliced

products

• Or repetitive sequence motifs

• Deletion or errors in transcript….

Can be tested by changing

probe target sequence… find the

missing regionSingle probe is used for detection

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ADVANTAGES

High specificity

Quality and quantity of RNA can be determined

Probes with partial

homology can be used

Membranes can be

stored and re-probed

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DIS-ADVANTAGES

Dis-advantages

Small number of genes can be

dealt at one time

Degradation by RNases

Use of harmful chemicalsLow sensitivity

Detection with multiple probes is

difficult

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Thank you