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The Journal of Neuroscience, June 1, 2003, 23(11):4401-4405
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Mouse NG2+ Oligodendrocyte Precursors Express mRNA for Proteolipid Protein But Not Its DM-20 Variant: A Study of Laser Microdissection-Captured NG2+ Cells
Ping Ye,1 Robert Bagnell,2,3 andA. Joseph D'Ercole1 1 Department of Pediatrics, The University of North Carolina at Chapel Hill, Chapel Hill, North Carolina 27599, 2 Department of Pathology and Laboratory Medicine, The University of North Carolina at Chapel Hill, Chapel Hill, North Carolina 27599, and 3 Department of Microscope Service Laboratory, The University of North Carolina at Chapel Hill, Chapel Hill, North Carolina 27599
Abstract
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Abstract
Introduction
Despite recent advances in our understanding of lineage of oligodendrocytes, detailed molecular characterization of this lineage in vivo is limited, primarily because of our inability to obtain a pure population of cells in situ. To define the molecular characteristics of oligodendrocyte lineage cells during development and their response to injury, we developed a strategy that uses laser capture microdissection (LCM) to isolate cells from sections and reverse transcription-PCR to determine mRNA expression. As a first step, we examined the expression of myelin-specific protein genes in NG2+ cells in cerebral cortex. We demonstrate that NG2+ cells in both developing and adult mice express NG2 mRNA but not mRNA for proteins specific for astrocytes, neurons, or microglia, indicating that a highly pure population of antigen-specific cells of the oligodendrocyte lineage can be obtained using LCM. Furthermore, we show that NG2+ cells express mRNAs for proteolipid protein (PLP), myelin basic protein, and 2',3'-cyclic nucleotide 3'-phosphodiesterase, but they dot not express DM-20 mRNA, a PLP mRNA splicing variant. Our data demonstrate that antigen-specific cells of oligodendrocyte lineage differentially express mRNA for myelin-specific proteins and their variants in vivo, partly define the gene expression in NG2+ cells, and raise questions about the cellular sites of DM-20 expression. This work also shows that LCM is a valuable tool to define and analyze gene expression in the cells of the oligodendrocyte lineage.
Key words: oligodendrocyte precursor; NG2; PLP; DM-20; MBP; gene expression; LCM
Introduction
In the CNS, oligodendrocytes develop from glial progenitors in the ventricular and subventricular zones (Hirano and Goldman, 1988; Levison and Goldman, 1993
To define the pattern of gene expression in the cells of the oligodendrocyte lineage during development and after injury, we developed a strategy that uses laser capture microdissection (LCM) to remove cells from sections. This allows isolation of RNA from defined in vivo cell populations and use of RT-PCR to precisely identify the mRNAs that they express. Here we report the expression of myelin protein genes in NG2 immunopositive (NG2+) cells in the cerebral cortex (CTX). We provide evidence that the NG2+ cells express mRNAs for proteolipid protein (PLP), MBP, and 2',3'-cyclic nucleotide 3'-phosphodiesterase (CNP) but not the mRNA for DM-20, a PLP mRNA splicing variant. Our data indicate that NG2 + cells are a unique population of cells in the oligodendrocyte lineage and that LCM is a valuable tool for defining and analyzing the molecular characteristics of antigen-specific cells in oligodendrocyte lineage in vivo.
Materials and Methods
Tissue collection. Under deep anesthesia, brains of mice (C57BL/6) were removed and collected. For whole CTX RNA extraction, CTX were dissected (n = 3) and frozen in liquid nitrogen. For immunohistochemistry and LCM, brains (n = 3) were split near the middle sagittal line, frozen in liquid nitrogen, and sagittally sectioned at a thickness of 8 µm on a cryostat. Both sections and CTX were stored at -80°C until use. All procedures used were approved by the institutional review committee of the University of North Carolina at Chapel Hill.Immunohistochemistry and cell capture. After thawing at room temperature briefly, sections near the midsagittal line were fixed with 75% ethanol for 20 sec and washed with PBS. In the presence of RNase inhibitor (200 U/ml; Promega, Madison, WI), the sections were immunostained for NG2 + cells for 30 min using an anti-NG2 antibody (1:400; a gift from Dr. Bill Stallcup, The Burnham Institute, La Jolla, CA). Antibody–antigen complexes were detected using peroxidase-conjugated polymers and visualized by incubation with DAB, provided in an EnVision+ immunostaining system (Dakocytomation; Dako, Carpinteria, CA).
After sections were dehydrated via a gradient concentration of ethanol, NG2 + cells (250–500) were microdissected and captured from two sections using a PixCell laser capture microdissector (Arcturus Engineering, Santa Clara, CA). Individual samples (250–500 NG2 + cells) derived from each brain were then transferred to a microcentrifuge tube containing 10 µl of cell lysis buffer provided in an RNA PicoPure kit (Arcturus Engineering).
Total RNA isolation and RT-PCR. Total RNA from NG2 + cells captured with LCM was extracted using the RNA PicoPure kit according the protocol of the manufacturer. Resultant RNA was dissolved in 10 µl of H2O and subjected to RT-PCR. Whole CTX RNA was isolated using the acidic guanidinium thiocyanate–phenol–chloroform method (Chomczynski and Sacchi, 1987
Sequence of cDNA derived from RT-PCR. PCR-amplified DNA fragments were resolved on 1% agarose gel. DNA band of interest was cut out and purified using Wizard PCR Preps DNA Purification System (Promega). DNA sequencing was performed at the Automated DNA Sequencing Facility at the University of North Carolina at Chapel Hill.
Southern blot hybridization analysis. PCR-amplified DNA fragments were fractionated on 1% agarose gel, transferred onto a nylon membrane, UV cross-linked, and hybridized with 32P-labeled single-stranded DNA (ssDNA) probe. PLP DNA fragment corresponding to bp 217–903 of mouse PLP cDNA (Hudson et al., 1987
Results
Consistent with previous reports (Nishiyama et al., 1997
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Figure 1. Representative microphotographs of a cerebral cortical section stained for NG2 + precursors derived from a 4-month-old mouse before (A) and after (B) LCM, as well as that of the same captured cells on a membrane (C). Arrows in A indicate NG2 + cells. Note that these cells are absent in B.
To confirm the identity of LCM-captured NG2+ cells and to determine whether there was contamination of captured NG2+ cells with other cell types, we used RT-PCR to examine the expression of mRNA derived from LCM-captured NG2+ cells derived from 4-month-old mice for the following cell-specific proteins: NG2, glial fibrillary acidic protein (GFAP)(astrocytes), CD68 (microglia–macrophages), and neurofilament light-subunit (NF-L) (neurons). Total RNA derived from whole CTX was used in parallel RT-PCR reactions. When CTX RNA was used, a single DNA band of the expected size was observed for each NG2, GFAP, CD68, and NF-L mRNA, respectively (Fig. 2). In contrast, only NG2 mRNA was detected in the LCM-captured cortical NG2+ cells, and no mRNA for GFAP, CD68, or NF-L mRNA was detected. These data show that LCM can be used to obtain NG2+ cells with little or no contamination of other CNS cell types.
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Figure 2. Expression of NG2, GFAP, CD68, and NF-L mRNAs in cerebral cortical NG2 + cells and whole cerebral cortex. Total RNA was isolated from LCM-captured NG2 + cells (LCM) and from whole cerebral cortex (CTX) of a 4-month-old mouse, and each RNA preparation was subjected to RT-PCR. RT-PCR DNA products were fractionated on 1% agarose gel containing ethidium bromide and photographed under UV light. The mRNA products derived from RT-PCR are indicated on the top of each lane.A DNA ladder of 100 bp markers was loaded in the left lane, and the size of the 400 and 600 bp bands are indicated by arrows. Note that the bands at bottom of the figure are primers used for RT-PCR.
Next, we examined the expression of mRNAs for the four major myelin-specific proteins: PLP, MBP, myelin-associated glycoprotein (MAG), and CNP in NG2+ cells. RNA derived from CTX of adult mice was again used as a control. mRNAs for all four myelin-specific proteins were detected in CTX RNA. As expected, multiple splicing forms of PLP, MBP, and MAG mRNA were clearly distinguished. As Figure 3A shows, two PLP bands of 582 and 687 bp representing DM-20 and PLP mRNA, respectively, were evident. Similarly, three MBP bands of 354, 422–442, and 479 bp (representing mRNA coded for 14, 17, or 18.5 kDa MBP, respectively) and two MAG bands
343 and 388 bp (coding for the large and small forms of MAG, MAG-L and MAG-S, respectively) were detected. Among these mRNA variants of each myelin protein gene, mRNA coding for 14 kDa MBP, PLP, and MAG-S was the most abundant, a finding consistent with previous studies showing that 14 kDa MBP, PLP, and MAG-S proteins and their mRNAs are predominately expressed in the CNS of adult mice (Morell et al., 1972
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Figure 3. Expression of myelin protein mRNA in cerebral cortical NG2 + cells and whole cerebral cortex. A, Expression of PLP, CNP, MAG, and MBP mRNAs in 4-month-old mice. Total RNA was isolated from LCM-captured NG2 +cells(LCM) and from whole cerebral cortex (CTX) of amouse and was subjected to RT-PCR.RT-PCR DNA products were separated on 1%agarose gel. Each mRNA product derived from RT-PCR is indicated on the top of each lane. B, Expression of PLP–DM-20 and MBP mRNA during development. Total RNA was extracted from cerebral cortical NG2 + cells (LCM) and cerebral cortex (CTX) of a 5-d-old mouse (P5) and a 4-month-old mouse (A), respectively, and subjected to RT-PCR. In both panels, DNA 100 bp markers were loaded in the middle lane.The arrowheads on the left of the panel indicate the expected sizes for RT-PCR amplified DNA derived from PLP (687 bp) and DM-20 (582 bp) mRNA, respectively. The arrowheads on the right indicate the expected sizes for RT-PCR amplified DNA (479, 422, and 354 bp) derived from MBP mRNA variants, respectively.
When RNA derived from LCM NG2+ cells was used, PLP and MBP mRNAs also were readily detected (Fig. 3A). RT-PCR amplification also identified a single faint CNP band and MAG bands. The MAG bands, although clearly visible on the gel under UV light, did not photograph well in Figure 3. In contrast to CTX RNA, which contained both PLP and DM-20 mRNAs, LCM NG2+ cells exhibited only one RT-PCR-amplified DNA band at 687 bp (i.e., the smaller 582 bp DM-20 band was not observed). To be certain that the 687 bp DNA band in LCM samples was derived from PLP mRNA, the DNA band was sequenced after gel purification. DNA sequencing data confirmed that the 687 bp band derived from isolated NG2+ cells corresponded to PLP mRNA (data not shown).
Three MBP 354, 422–442, and 479 bp bands (corresponding to MBP mRNA splicing variants coding for 14, 17, and 18.5 kDa proteins, respectively) also were observed in RNA from NG2+ cells. Unlike adult CTX that expresses predominately mRNA encoded for 14 kDa MBP, however, mRNA for 18.5 kDa MBP (the 479 bp band) was the most abundant form in NG2+ cells.
DM-20 mRNA has been shown to be the predominant form of the two PLP isoforms during early development (Morell et al., 1972
The expression of MBP mRNA in the NG2+ cells of P5 CTX also was examined. Unlike adult CTX, which expresses predominately mRNA coding 14 kDa MBP (354 bp band), mRNAs encoding larger MBP isoforms (17 and 18.5 kDa, i.e., the 422–442 and 479 bp bands, respectively) were more abundant in the NG2+ cells, findings that are consistent with those that we observed in RNA derived from adult NG2+ cells.
To exclude the possibility that DM-20 mRNA is expressed at low levels in NG2+ cells, two rounds of PCR amplification for PLP–DM-20 mRNA from both P5 and adult mice were performed, followed by Southern blot hybridization analysis using a 32P-labeled PLP probe that hybridizes both PLP and DM-20 cDNA. In multiple experiments, we were unable to detect DM-20 mRNA in cortical NG2+ cells derived from P5 or adult mice. A representative PLP Southern hybridization blot is shown in Figure 4.
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Figure 4. Representative Southern blot hybridization analysis of RT-PCR amplified PLP–DM-20. A, RT-PCR amplified PLP–DM-20 DNA fragments derived from cerebral cortical NG2 + cells (LCM) and cerebral cortex (CTX) of a 5-d-old mouse (P5) and a 4-month-old mouse (A) were fractionated on 1% agarose gel. B, DNA fragments, fractionated on 1% agarose shown in A, were transferred onto a nylon membrane, hybridized with a 32P-labeled PLP ssDNA probe, and exposed to an x-ray film for
Discussion
Using LCM, we demonstrated that it is possible to isolate a population of NG2+ cells from mouse CTX sections with little or no contamination of microglia, astrocytes, or neurons. We showed that NG2+ cell RNA contains mRNAs specific for NG2 and several myelin-specific proteins, including PLP and MBP, but not mRNAs for other cell type-specific proteins, such as GFAP (astrocytes), NF (neurons), and CD68 (microglia). These findings are consistent with previous data showing that NG2+ cells do not react with the antibodies specific for astrocytes, neurons, or microglia (Nishiyama et al., 1997NG2 is a large cell surface proteoglycan that is expressed in the CNS of both developing and adult rodents and humans (for review, see Dawson et al., 2000
R and A2B5 in vivo and in culture (Stallcup and Beasley, 1987
In adult rodents, NG2+ cells also are abundant in the CNS (Nishiyama et al., 1996
Our findings that PLP, but not DM-20, mRNA is detected in NG2+ oligodendrocyte precursors during development are consistent with those of Mallon et al. (2002
DM-20 mRNA and its protein, products of an alternatively spliced PLP mRNA that lacks 105 nucleotides in the exon 3 (Nave et al., 1987
In summary, using LCM in combination with RT-PCR, we demonstrated that CNS NG2+ cells express only PLP mRNA and not the DM-20 isoform. These data offer new insights into the gene expression of cells in the oligodendrocyte lineage. Our data also demonstrate that LCM methodology is a powerful tool to investigate the molecular characteristics of single antigenic positive cells in vivo.
Footnotes
Received Jan. 15, 2003; revised Feb. 28, 2003; accepted Mar. 13, 2003.This work was supported by National Institutes of Health Grant NS38891 (National Institute of Neurological Disorders and Stroke) to A.J.D. We thank Dr. Pierer Morell for critical reading of this manuscript and helpful discussion.
Correspondence should be addressed to Dr. Ping Ye, Department of Pediatrics, CB 7039, The University of North Carolina at Chapel Hill, Chapel Hill, NC 27599-7220. E-mail: ping_ye{at}med.unc.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/234401-05$15.00/0
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