RNA Detection

LE probe contains two regions: region I on 3^0 -end hybri-

dizes with adaptor probe and region II on 5^0 -end has com-

plementary sequence with target RNA. A “TTTTT”

sequence is inserted between the two regions.

l A1 5^0 ACA CAGAA AGG GAA ACGAGTCC CGT

TTC CCT TTC.

l A2 5^0 CGT TTC CCT TTCTGTGTGAA AGG GAA

ACGGGA CT.

l X1* 5^0 CGT TTC CCT TTCTGT GTTTTTTATA TCC

CTC GCC GAA TCC TAG ACTCAAAGTAGT CTA

GGA TTC GGC GAG.

X1*^0 consists of two regions: region I on 3^0 -end has the same

sequence with probe X1 and region II on 5^0 -end is a hangout

branch that can initiate the polymerization of hairpin set A.

A “TTTTT” sequence is inserted into the two regions.

l X2 5^0 AGT CTA GGA TTC GGC GAGGGATATCTC

GCC GAA TCC TAG ACTACT TTG.

l Italic sequence indicates the toehold region, bold typeface

indicates loop sequences, and underline indicates stem

sequences.

15. Target oligo: 5^0 AGT CTA GGA TTC GGC GAGGGATAT
    TTTTT CTC TTG GAA AGA AAG TG.
    The target oligo can hybridize on its 3^0 -half with the capture
    probe on a solid support; the 5^0 -half of “Target oligo” can
    initiate the polymerization of hairpin set X*. A “TTTTT”
    sequence is inserted between the two regions.


16. Adaptor: AGT CTA GGA TTC GGC GAGGGA TATTTTTT
    ATG CTT TGA CTC AGA AAA CGG TAA CTT C.


17. 4
    SYBR Green I: dilute with 4
    SSC before use, store at 4C
    (seeNote 5).

3 Methods

Carry out all procedures at room temperature unless otherwise

specified.

3.1 Preparation 1. All hairpin probes are heated to 95C for 2 min and then
allowed to cool to room temperature for 1 h before use.

3.2 Linear HCR by
1.5% Agarose Gel
Electrophoresis

1. Mix 7μL of water, 1μL of probe A1, and 1μL of probe A2,
   1 μL of target with different concentrations and 1μL of water
   for control, incubate at room temperature for 4 h.

192 Yao Xu and Zhi Zheng