RCA Protocol: Direct RNA Strategy¶

This is the direct RNA library construction protocol shared by all sample types (FF, FFPE) and readout technologies (PRISM, SPRINTseq). Padlock probes hybridize directly to mRNA, and SplintR ligase ligates the DNA nick on the RNA template. Start here after completing sample pre-treatment (Fresh Frozen or FFPE).

cDNA strategy

For the cDNA ligation strategy (reverse transcription before hybridization, with T4 DNA Ligase for SNP specificity), see RCA Protocol: cDNA.

Version: v5.3
Last modified: 2026-01-29

1. Blocking (~30 min)¶

Goal: Block nonspecific sites.

Reagent	Stock	Final	100 μl
RNase Free H₂O			58.5 μl
Ampligase Buffer	10X	1X	10 μl
KCl	1 M	0.05 M	5 μl
Formamide	100%	20%	20 μl
Oligo dT	100 μM	1 μM	1 μl
Recombinant Albumin	20 μg/μl	0.2 μg/μl	1 μl
tRNA	10 μg/μl	0.2 μg/μl	2 μl
RiboLock	40 U/μl	1 U/μl	2.5 μl

Incubate: Add Blocking Mix, incubate at RT for 30 min.

2. Hybridization (~2.5 h)¶

Goal: Probe-specific binding.

Probe volume

Probe stock concentration and volume depend on the specific probe panel. Adjust to achieve the desired final concentration (typically 0.05--0.2 μM per probe). Fill H₂O to 100 μl total.

Reagent	Stock	Final	100 μl
RNase Free H₂O			to 100 μl
Ampligase Buffer	10X	1X	10 μl
KCl	1 M	0.05 M	5 μl
Formamide	100%	20%	20 μl
Probes	(panel-dependent)	0.05--0.2 μM	(variable)
Recombinant Albumin	20 μg/μl	0.2 μg/μl	1 μl
tRNA	10 μg/μl	0.2 μg/μl	2 μl
RiboLock	40 U/μl	1 U/μl	2.5 μl

Incubate: 55°C (15--20 min denaturation) → 45°C (120 min hybridization). Seal to prevent evaporation.
Stringent Wash: 10% Formamide in 2X SSC, 3 x 10 min (45°C optimal, or RT). Washing buffer: 100 µL 20X SSC + 100 µL formamide + 800 µL NFW.
Wash: PBS-Tween 0.05% wash 2--3 x 1 min (remove residual formamide to avoid deactivating ligase).

3. Ligation (~2 h)¶

Goal: Ligation of hybridized padlock probes into circles; SplintR ligase (PBCV-1 DNA Ligase) works on DNA:RNA hybrids.

Reagent	Stock	Final	100 μl
RNase Free H₂O			76.5 μl
SplintR Buffer	10X	1X	10 μl
Recombinant Albumin	20 μg/μl	0.2 μg/μl	1 μl
SplintR Ligase	25 U/μl	2.5 U/μl	10 μl
RiboLock	40 U/μl	1 U/μl	2.5 μl

Incubate: 37°C for 2 hours (sealed).
Wash: PBS-Tween 0.05% wash 2 x 1 min.

4. Rolling Circle Amplification (~12--16 h)¶

Goal: Amplify circularized probes into DNA nanoballs (rolonies).

Reagent	Stock	Final	100 μl
RNase Free H₂O			63.5 μl
Phi29 Buffer	10X	1X	10 μl
Glycerol	100%	~10%	10 μl
dNTPs	10 mM	0.25 mM	2.5 μl
Amino-dUTP	2 mM	50 μM	2.5 μl
Recombinant Albumin	20 μg/μl	0.2 μg/μl	1 μl
RCA Primer	10 μM	0.3 μM	3 μl
Phi29 Polymerase	10 U/μl	0.25 U/μl	2.5 μl
RiboLock	40 U/μl	1 U/μl	2.5 μl

Incubate: 30°C for 12--16 h overnight (sealed / humid chamber).
Wash: PBS-Tween 0.05% wash 2 x 1 min.

5. Post-amplification Fix & Strip¶

Goal: Fix RCA products and strip unbound probes.

Fix: Add 4% PFA, mix by gentle pipetting (3--5 times), incubate 15--30 min at RT.
Wash: PBS-Tween 0.05% wash 3 x 1 min.
Strip: 65% formamide wash 3 x 2--10 min at 30°C (e.g. on a PCR block or Eppendorf Thermostat). Washing buffer: 650 µL formamide + 350 µL NFW.
Wash: PBS-Tween 0.05% wash 2 x 1 min.

Autofluorescence Quenching (Optional)¶

When to use

This step is optional and depends on sample autofluorescence. FFPE samples almost always require it. Some FF samples (e.g. tissues with high lipofuscin content) may also benefit. Perform before signal readout (PRISM imaging or SPRINTseq sequencing).

Sudan Black B:

Stock solution: 0.1% (wt/vol) Sudan Black B in 70% EtOH (e.g. 10 mg in 10 ml). Shake at RT for days, filter before use.

Incubate: RT for 10 min.
Wash: 70% EtOH wash 10 x 3 min.
Wash: PBS-Tween 0.05% wash 2 x 1 min.

Warning

Sudan Black B may reduce signal intensity. Test on control samples first.

Next step: Signal readout -- PRISM Imaging or SPRINTseq Sequencing