MicroRNA In situ Hybridization for Formalin Fixed Kidney Tissues

Summary

This article describes an in situ hybridization protocol optimized for colormetric detection of microRNA expression in formalin fixed kidney sections.

Abstract

In this article we describe a method for colorimetric detection of miRNA in the kidney through in situ hybridization with digoxigenin tagged microRNA probes. This protocol, originally developed by Kloosterman and colleagues for broad use with Exiqon miRNA probes¹, has been modified to overcome challenges inherent in miRNA analysis in kidney tissues. These include issues such as structure identification and hard to remove residual probe and antibody. Use of relatively thin, 5 mm thick, tissue sections allowed for clear visualization of kidney structures, while a strong probe signal was retained in cells. Additionally, probe concentration and incubation conditions were optimized to facilitate visualization of microRNA expression with low background and nonspecific signal. Here, the optimized protocol is described, covering the initial tissue collection and preparation through the mounting of slides at the end of the procedure. The basic components of this protocol can be altered for application to other tissues and cell culture models.

Introduction

MicroRNA are small (approximately 22 nucleotides long) noncoding RNAs that are endogenously produced. They generally function to suppress protein expression through translational repression or mRNA degradation. miRNAs bind to mRNA targets with incomplete complementarity, making it possible for a single miRNA to suppress multiple targets.

Understanding which cell types and structures express miRNAs is an important part of understanding the mechanisms through which alterations in miRNA expression influence cell and tissue phenotypes. While methods such as miRNA sequencing, qPCR and Northern blotting can be used for detection of miRNAs in whole tissues, this approach does not allow one to determine which specific cell type they came from within a given tissue. Dissection of cellular and structural components prior to analysis using these methods can be very difficult and the conditions needed to achieve adequate isolations can lead to alterations in gene expression or degradation of RNAs. microRNA in situ hybridization is a method used to visualize microRNA location and expression levels in tissues. This technique is especially valuable in tissues composed of heterogeneous structures, such as the kidney.

MicroRNAs have been shown to play an regulatory role in kidney development^2,3 and physiology⁴. microRNA expression alterations have also been shown to be involved with renal pathology such as fibrosis^5-10, diabetic nephropathy⁷, renal carcinoma^11,12, and acute kidney injury¹³. In our research, we have found that optimizing microRNA in situ hybridization for kidney tissues was valuable for determining the exact structural locations of miRNA expression in both health and disease¹⁴. Determination of the tubular and cellular expression of different microRNAs is important because their regulation of targets may be dependent on cellular functions. In diseased states it is also important to determine how alterations in miRNA expression may be impacting function.

The goal of the method described here was to build upon existing ISH methodologies developed by Kloosterman et al.¹⁵, other investigators^16,17, and those suggested by Exiqon¹ and optimize the method for formalin fixed kidney tissues. We have successfully used this method to identify distinct regional differences in renal microRNA miR-382 expression with unilateral ureteral obstruction¹⁸. This approach can be used with other tissues as well, with additional optimization.

Protocol

1. Kidney Tissue Sections

1. Formalin-fixed (10%) paraffin-embedded kidney sections are cut onto microscope slides at 5 mm thickness using a Microm HM 355 S. The slides can be stored for several months before analysis.

2. Solution Preparation

1. Prepare 1 L of 1x PBS in ddH₂O in an autoclavable screw top bottle. Fill another bottle with 1 L of ddH₂O. Add 1 ml of DEPC to each bottle, cover and shake vigorously. Let the solutions sit overnight at room temperature to destroy RNAses and then autoclave. Add 400 ml Tween-20 to 1 L of 1x PBS to make PBS-T.
2. Prepare proteinase K buffer (50 mMTris-HCl, pH 8.0 and 1 mM CaCl₂ in DEPC treated water).
3. Prepare a solution of 0.2% glycine in PBS-T.

3. Tissue Preparation

1. Prepare a large volume of hybridization buffer (50-100 ml) composed of 50% Formamide, 5x SSC, 0.1% Tween, 9.2 mM citric acid for adjustment to pH 6, 50 µg/ml heparin, and 500 µg/ml yeast RNA in DEPC treated ddH₂O. Divide into 1 ml aliquots and store at -80 ºC.
2. Remove the paraffin from the tissue by washing 3x in fresh xylene for 5 min each.
3. Rehydrate the tissue sections by 5 min incubations in decreasing concentrations of ethanol (100%, 75%, 50%, and 25%) in ddH₂O.
4. Treat the slides with enough DEPC to completely cover the tissue sections (approximately 0.4-0.5 ml) for 1 min. Make sure tissues do not dry out.
5. Rinse the slides in DEPC treated PBS-T twice for 5 min, collecting the DEPC containing waste for proper disposal. All reagents should be DEPC treated to eliminate RNAses from this point on.
6. Prewarm Proteinase K buffer and add proteinase K to a final concentration of 10 μg/ml. Cover tissue sections with proteinase K solution and incubate at 37 ºC for 5 min.
7. Quickly remove the proteinase K solution and add 0.2% glycine in PBS-T for 30 sec.
8. Rinse slides in DEPC treated PBS-T twice for 30 sec each.
9. Fix sections in freshly made 4% paraformaldehyde for 10 min.

4. Hybridization

1. Add 50 µl of hybridization buffer (50% Formamide, 5x SSC, 0.1% Tween, 9.2 mM citric acid for adjustment to pH 6, 50 µg/ml heparin, 500 µg/ml yeast RNA) per tissue section and cover with RNAse free HybriSlips cut just larger than the tissue sections.
2. Prehybridize sections in humidity controlled hybridization oven for 2 hr at hybridization temperature determined for the 3’ digoxigenin labeled probe (usually DNA Tm of the probe -21 °C, ( i.e. 54 °C for miR-382, probe DNA Tm= 75 °C), using tissue lab wipes soaked in 50% formamide/50% 5x SSC to keep the chamber humidified.
3. Dilute the miRNA probe, positive control (U6, small nuclear RNA) and negative control (scrambled sequence) to 40 nM in hybridization buffer (75 µl of buffer is needed per section).
4. Heat the probe in hybridization buffer at 65 ºC for 5 min.
5. Remove slides from hybridization oven and remove coverslips and excess hybridization buffer from prehybridization.
6. Add 75 µl of probe containing buffer per tissue section, directly to tissue. Cover tissue with HybriSlips just large enough to cover the tissue sections.
7. Keeping slide holder level, return to hybridization oven for overnight incubation at temperature from step 4.2 (approximately 16 hr).

5. Stringency Wash

1. Add 200 µl 2x SSC, heated to the hybridization temperature, just under one edge of the coverslips to help release the coverslip from the tissue. Remove the coverslip by tilting the slide.
2. Wash the slides in 200 µl of 50% formamide, 50% 2x SSC at hybridization temperature 3x for 30 min each.
3. Rinse the slides 5x in PBS-T at room temperature for 5 min each on orbital shaker on low speed.

6. Detection

1. Incubate slide in blocking buffer (2% goat or horse serum, 2 mg/ml BSA in PBS-T) for 1 hr at room temperature on orbital shaker on low speed.
2. Dilute anti-DIG-AP Fab fragments in blocking buffer at 1:100. Add 100 µl per tissue section and cover with HybriSlips cut just large enough to cover the section.
3. Incubate antibody in a humidified chamber at 4 °C overnight (approximately 16 hr).
4. Wash the slides in PBS-T 7x, for 5 min each on orbital shaker at low speed.
5. Wash the slides in AP buffer (100 mM TrisHCl pH 9.5, 50 mM MgCl₂,100mM NaCl, 0.1% Tween 20) 3x, for 5 min each.
6. Add NBT/BCIP solution to AP buffer (200 µl/10 ml buffer)
7. Add 400-500 ml of diluted NBT/BCIP solution to each slide to completely cover all tissue sections. Develop in a dark, level, humidified chamber for 4-5 hr.

7. Mounting Slides

1. Dehydrate sections in increasing concentrations of ethanol (25%, 50%, 75%, 100%) for 5 min each.
2. Incubate in xylene 5x in order to clear sections.
3. Mount slides in Permount mounting medium and dry overnight.

Results

The areas of a tissue section that become dried out during the hybridizations, incubations or wash steps generally end up staining more darkly during the NBT/BCIP development. Figure 1 shows a portion of a kidney section in which the HybriSlip slipped off of the edge of the tissue, allowing it to become partially dehydrated. Despite rehydration and coverage in the remaining steps, the signal in the dehydrated portion is artificially high.

The importance of controlling the time...

Discussion

The goal of this article was to describe a protocol for miRNA in situ hybridization that works well in formalin fixed kidney tissues. While working out this protocol several important sources of staining artifact have been identified. Careful attention to these points can help avoid staining artifact and increase the likelihood of a successful ISH run.

One of the most avoidable causes of staining artifact can occur when tissue sections become dried out during long incubations. When th...

Materials

Name	Company	Catalog Number	Comments
Paraformaldehyde	Sigma	P6148
PBS	Gibco	70011044
Diethyl Pyrocarbonate	Sigma	D5758
Tween-20	Sigma	P1379
Xylenes	Sigma	534056
Ethanol	Ultra Pure	200CSPTP
Tris-HCl	Life Technologies	15506-017
CaCl2	Sigma	C2536
Glycine	J.T. Baker	4059-00
Citric Acid	Sigma	C2404
Formamide	Sigma	F9037
20x SSC Buffer	Life Technologies	15557-044
Heparin	SAGENT	25021-400-30
Yeast RNA	Life Technologies	AM7118
MgCl2	Sigma	M8266-1004
NaCl	J.T. Baker	4058-01
Proteinase K	Fermentas	EO0491
3’ DIG- miRNA probe	Exiqon	miR dependent-05
3’ DIG- Scrambled miR probe	Exiqon	99004-05
3’ DIG- U6 miR probe	Exiqon	99002-05
Anti-Digoxigenin-Ab Fab	Roche	11093274910
NBT/BCIP	Roche	11681451001
Permount	Fisher	SP15-500
Coverslips	Fisher	Fit to tissue size
Microtom HM 355 S	Thermo Scientific	23-900-672
In-slide Out Hybridization Oven	Boekel	241000
Aluminum Tray Assembly	Boekel	C2403973
Stainless Steel Rack Insert	Boekel	C2403754