DNA/RNA extraction from fresh-frozen tissue, AllPrep DNA/RNA/miRNA Universal Kit

Annika Fendler

Published: 2023-07-03 DOI: 10.17504/protocols.io.kxygx3mrwg8j/v2

DNA

RNA

Fresh-frozen tissue

Qiagen AllPrep

AI 解读

Abstract

Protocol for combined RNA and DNA extraction from fresh-frozen tissue using the AllPrep DNA/RNA/miRNA Universal Kit.

Before start

Preparations:

FRN buffer: Add 42 ml Isoprop to new bottle

RPE buffer: Add 44 ml EtOH to new bottle

AW1 buffer: Add 25 ml EtOH to new bottle

AW2 buffer: Add 30 ml EtOH

DNAse I stocks: 550 µl RNase-free water to lyophilised DNAse I, aliquot and store at -20°C for 9 months)

Immediately

DNAse I: 70 µl RDD + 10 µl DNase I per sample

Proteinase K: 60 µl AW1 + 20 µl Proteinase K per sample

Steps

Tissue preparation

This protocol is for Sample

Optional: Weigh tissue

Enter a complete list of samples used for each experiment below:

A	B	C

List of tissue sample used in experiment

Transfer tissue in 350µL 600µL RLT + ß-ME in 2 ml DNA LoBind tube.

Make sure that the tissue does not defrost.

Add a 5mm bead to each tube and lyse tissue in TissueLyser for 0h 2m 0s @ 20 Hz

Equipment

Value	Label
TissueLyser II	NAME
Bead Mill	TYPE
QIAGEN	BRAND
85300	SKU

Spin down for 0h 1m 0s @ 9000x g,0h 0m 0s

Turn tube rack and lyse tissue for 0h 2m 0s @ 20 Hz

Spin down for 0h 1m 0s @ 9000x g,0h 0m 0s

Add lysed product to DNA Mini Spin Column

Spin 0h 0m 30s @ maxx g,0h 0m 0s , repeat if any liquid remains on column

Transfer column to a new collection tube and store tube at 4°Cuntil DNA extraction

10.

Transfer flow-through to new 2 ml LoBind tube

RNA extraction

11.

Add 50µL 80µL Proteinase K, mix by pipetting

12.

Add 200µL 350µL EtOH abs., mix by inverting, spin down liquid

13.

Incubate 0h 10m 0s @ Room temperature

14.

Add 400µL 750µL EtOH abs. , mix by pipetting

15.

Add 700µL to RNeasy spin column and spin for 0h 0m 30s @ maxx g,0h 0m 0s and discard flow-through

16.

Repeat until all liquid passed through the column

17.

Add 500µL RPE

18.

Spin 0h 0m 30s @ maxx g,0h 0m 0s and discard flow-through

19.

Add 80µL DNase I working solution directly onto the membrane and incubate 0h 15m 0s at Room temperature

20.

Add500µL FRN

21.

Spin 0h 0m 30s @ maxx g,0h 0m 0s and don't discard flow-through

22.

Add flow-through again to column

23.

Spin 0h 0m 30s @ maxx g,0h 0m 0s and discard flow-through

24.

Add 500µL RPE

25.

Spin 0h 0m 30s @ maxx g,0h 0m 0s and discard flow-through

26.

Add 500µLEtOH abs

27.

Spin 0h 2m 0s @ maxx g,0h 0m 0s and place column in new collection tube

28.

Spin 0h 2m 0s @ maxx g,0h 0m 0s and place column in new 1.5 ml collection tube

29.

Add 30µLof RNase-free H₂O

30.

Incubate 0h 1m 0s @ Room temperature

31.

Spin down0h 1m 0s @ 8000x g,0h 0m 0s

32.

QC: Qubit and tape station

32.1.

Citation

Upload PDF from Tapestation here

DNA extraction

33.

350µL AW1 auf DNA Mini Spin Column geben

34.

Spin 0h 0m 30s @ maxx g,0h 0m 0s and discard flow-through

35.

80µLProteinase K working solution directly onto membrane

36.

Incubate 0h 5m 0s @ Room temperature

37.

Add 350µL AW1

38.

Spin 0h 0m 30s @ maxx g,0h 0m 0s and discard flow-through

39.

Add 350µL AW2

40.

Spin 0h 2m 0s @ maxx g,0h 0m 0s and place column in new 2 ml collection tube

41.

Spin 0h 1m 0s @ maxx g,0h 0m 0s and place column in new 1.5 ml collection tube

42.

Add 50µL directly onto membrane

43.

Incubate 0h 1m 0s @ Room temperature

44.

Spin down 0h 1m 0s @ 8000x g,0h 0m 0s

45.

QC: Qubit DNA and tape station

45.1.

Citation

Note

Upload Tapestation results as pdf here

50.

Inferring cellular and molecular processes in single-cell data with non-negative matrix factorization using Python, R and GenePattern Notebook implementations of CoGAPS

DNA/RNA extraction from fresh-frozen tissue, AllPrep DNA/RNA/miRNA Universal Kit

Abstract

Before start

Steps

Tissue preparation

RNA extraction

DNA extraction

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