Isolation of RNA from Acute Ischemic Stroke Clots Retrieved by Mechanical Thrombectomy

Vincent M Tutino; Sarah Fricano; Kirsten Frauens; Tatsat R Patel; Andre Monteiro; Hamid H Rai; Muhammad Waqas; Lee Chaves; Kerry E Poppenberg; Adnan H Siddiqui

doi:10.3390/genes12101617

Isolation of RNA from Acute Ischemic Stroke Clots Retrieved by Mechanical Thrombectomy

Genes (Basel). 2021 Oct 14;12(10):1617. doi: 10.3390/genes12101617.

Authors

Vincent M Tutino^{1

2

3

4}, Sarah Fricano^{1

2}, Kirsten Frauens^{1

3}, Tatsat R Patel^{1

4}, Andre Monteiro^{1

3}, Hamid H Rai^{1

3}, Muhammad Waqas^{1

3}, Lee Chaves^{1

3}, Kerry E Poppenberg^{1

3}, Adnan H Siddiqui^{1

3

5}

Affiliations

¹ Canon Stroke and Vascular Research Center, University at Buffalo, Buffalo, NY 14203, USA.
² Department of Pathology and Anatomical Sciences, University at Buffalo, Buffalo, NY 14260, USA.
³ Department of Neurosurgery, University at Buffalo, Buffalo, NY 14260, USA.
⁴ Department of Mechanical & Aerospace Engineering, University at Buffalo, Buffalo, NY 14260, USA.
⁵ Department of Radiology, University at Buffalo, Buffalo, NY 14260, USA.

Abstract

Mechanical thrombectomy (MT) for large vessel acute ischemic stroke (AIS) has enabled biologic analyses of resected clots. While clot histology has been well-studied, little is known about gene expression within the tissue, which could shed light on stroke pathophysiology. In this methodological study, we develop a pipeline for obtaining useful RNA from AIS clots. A total of 73 clot samples retrieved by MT were collected and stored in RNALater and in 10% phosphate-buffered formalin. RNA was extracted from all samples using a modified Chemagen magnetic bead extraction protocol on the PerkinElmer Chemagic 360. RNA was interrogated by UV-Vis absorption and electrophoretic quality control analysis. All samples with sufficient volume underwent traditional qPCR analysis and samples with sufficient RNA quality were subjected to next-generation RNA sequencing on the Illumina NovaSeq platform. Whole blood RNA samples from three patients were used as controls, and H&E-stained histological sections of the clots were used to assess clot cellular makeup. Isolated mRNA was eluted into a volume of 140 µL and had a concentration ranging from 0.01 ng/µL to 46 ng/µL. Most mRNA samples were partially degraded, with RNA integrity numbers ranging from 0 to 9.5. The majority of samples (71/73) underwent qPCR analysis, which showed linear relationships between the expression of three housekeeping genes (GAPDH, GPI, and HPRT1) across all samples. Of these, 48 samples were used for RNA sequencing, which had moderate quality based on MultiQC evaluation (on average, ~35 M reads were sequenced). Analysis of clot histology showed that more acellular samples yielded RNA of lower quantity and quality. We obtained useful mRNA from AIS clot samples stored in RNALater. qPCR analysis could be performed in almost all cases, while sequencing data could only be performed in approximately two-thirds of the samples. Acellular clots tended to have lower RNA quantity and quality.

Keywords: RNA extraction; RNA sequencing; acute ischemic stroke; large vessel occlusion; method; quantitative polymerase chain reaction.

Publication types

Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov't

MeSH terms

Acute Disease
Aged
Female
Humans
Ischemic Stroke / complications*
Male
RNA / isolation & purification*
Real-Time Polymerase Chain Reaction / methods
Thrombectomy / methods*
Thrombosis / etiology
Thrombosis / surgery*

Substances

RNA

Abstract

Publication types

MeSH terms

Substances

Grants and funding