(Received for publication, May 23, 1995; and in revised form, July 5, 1995)
From the
Rat preosteoblastic cells, UMR201, develop a more mature phenotype when subcultured onto a type I collagen gel when compared with their growth on plastic. Basal osteopontin mRNA expression is up-regulated, whereas retinoic acid-induced alkaline phosphatase expression is reduced in cells on collagen when compared with cells plated onto plastic. We have used differential display polymerase chain reaction (PCR) of mRNA to identify other mRNA species that are regulated by collagen and/or retinoic acid in UMR201 cells. A number of differentially expressed PCR products were isolated, whose sequences did not correspond to known sequences in the data bank. However, one species which was up-regulated by growth on collagen showed 95 and 94% homology to the murine and canine 54-kDa subunit of the signal recognition particle (SRP54), respectively. In time course experiments, using reverse transcription PCR, it was found that SRP54 mRNA was up-regulated in UMR201 cells as early as 1 h after subculture onto collagen, when compared with cells subcultured onto plastic, and levels remained elevated after 48 h. The increased expression of SRP54 paralleled the increased expression of a known secreted protein, osteopontin. SRP54 recognizes signal sequences of proteins destined for secretion and retards them for further elongation in the endoplasmic reticulum. The increased expression may correlate with the synthesis of specific extracellular matrix molecules in differentiating osteoblasts.
It is well recognized that the extracellular matrix environment
can regulate gene expression of cells in a tissue-specific manner (for
review, see (1) ). Differentiation has been demonstrated in
mammary gland epithelial cells cultured onto either type I collagen
gels or a reconstituted basement membrane material(2) , in
hepatocytes cultured on a basement membrane-like matrix (3) or
laminin(4) , in sertoli cells cultured onto laminin-rich
substrata(5, 6) , and more recently in bone cells
cultured onto type I collagen(7, 8) . We have shown
that the preosteoblastic cells, UMR201(9) , were directed to a
more mature phenotype when cells were plated onto a matrix of gelled
type I collagen(7) . Growth on type I collagen was shown to
decrease growth rate, down-regulate RA()-stimulated alkaline
phosphatase mRNA and enzyme levels, as well as increase the basal and
RA-stimulated expression of OP. Alkaline phosphatase and OP are among
the genes whose expression is known to be modulated during osteoblast
differentiation(10, 11, 12) . Since previous
studies from our group have demonstrated that plating cells on a
collagen substratum gave definitive and reproducible changes (7) in the differentiation profile of rat osteoblastic cells,
we used differential display-polymerase chain reaction (dd-PCR) to
identify other genes whose expression is regulated either by collagen
substratum and/or RA. The technique of differential display of mRNA
species (13) has recently been used to determine differentially
regulated mRNA species between comparative populations of
cells(14) , tissues(15) , and tumors(16) .
Using this technique, we have identified a regulated mRNA species that codes for a protein involved in the protein secretory pathway. Most proteins destined for secretion first pass through the endoplasmic reticulum (for reviews, see refs. 17-19). Identification and targeting of nascent polypeptide chains is apparently achieved by the binding of the 54-kDa subunit of the signal recognition particle (SRP54). Evidence suggests that SRP54 binds to the signal sequence as it emerges from the ribosome, thereby forming a complex and retarding further elongation of the polypeptide chain. This ribosome-SRP complex then binds to the SRP receptor on the endoplasmic reticulum membrane. The ribosome forms a complex with the ``translocon,'' translation elongation resumes, and SRP54 is released for another round of targeting(17, 19) . The regulation of this mRNA species has not been reported previously. We have identified a 267-bp sequence of the rat homologue of SRP54 using dd-PCR and show that this mRNA species was up-regulated when preosteoblastic cells, UMR201, were plated on a physiological substratum. The up-regulation of this mRNA species may be related to the differentiation state of the preosteoblasts. A more differentiated state of these cells in response to plating on type I collagen is demonstrated with concomitant up-regulation of OP mRNA, a secreted protein which is a recognized marker of osteoblast differentiation.
The rat preosteoblast cell line, UMR201(9) , was used
in all experiments as described previously(7) . Briefly, cells
were routinely grown in -modified minimal essential medium
(
-MEM) (Life Technologies, Inc.) containing 10% fetal bovine serum
(Cytosystems, Castle Hill, New South Wales, Australia). All media
contained gentamicin (80 mg/ml) (David Bull Laboratories, Mulgrave,
Victoria, Australia) and minocycline (1 mg/ml) (Sigma). Incubations
were carried out at 37 °C and equilibrated with 5% CO
in humidified air. Cells were used between passages 9 and
11(9) . Cells on plastic were harvested using
phosphate-buffered saline with 5 mM EDTA. All chemicals were
purchased from BDH (Kilsyth, Victoria, Australia) unless otherwise
specified.
Rat tail type I collagen (>99% purity; Collaborative
Research, Waltham, MA) gels were prepared resuspended in serum-free
-MEM at a concentration of 25 µg/cm
, as described
previously (7) . Human fibronectin (99% purity), murine laminin
(>94%), and human vitronectin (Collaborative Research) were used at
concentrations of 1, 1, and 0.1 µg/cm
, respectively,
resuspended in serum-free
-MEM supplemented with 1% bovine serum
albumin (to block nonspecific binding sites) to coat tissue culture
dishes. The concentrations used were in the range recommended by the
manufacturer. Isolation of RNA from cells grown on type I collagen
required matrix dissolution, which was achieved using 0.05% (w/v)
collagenase (Worthington) in phosphate-buffered saline at 37 °C for
20-30 min as described previously(7) .
Cells were
subcultured onto 170 cm plastic tissue culture dishes
(Becton Dickinson, Lincoln Park, NJ) that were either uncoated or
coated with matrix. Cells were plated at the appropriate density to
reach confluence at the time of RNA harvesting and grown in the
presence or absence of 1 µM RA for 1, 2, 6, 8, and 24 h.
RA was added at the time of subculture, and in the presence of fetal
bovine serum, almost all cells adhered to either plastic or collagen
within 1 h. Total RNA was extracted using guanidinium hydrochloride as
described (20) . For Northern analysis, 20 µg of total RNA
was loaded per lane of 1.2% (w/v) formaldehyde-agarose gels and
transferred to nylon filters (Amersham International, Buckinghamshire,
United Kingdom) following electrophoresis(21) . Complementary
DNA (cDNA) probes were nick-translated with
[
-
P]dCTP (Amersham) to a specific activity
of 1
10
dpm/µg DNA, according to the
manufacturer's specifications (Boehringer Mannheim, GmbH,
Mannheim, Germany). Specifically bound probe was quantified by
PhosphorImager analysis (Molecular Dynamics, Sunnyvale, CA).
Complementary DNA probes used were rat osteopontin (22) and chicken glyceraldehyde-3-phosphate dehydrogenase (GAPDH)(23) , the latter used to normalize mRNA species for loading variations.
The method of differential display of mRNA used was essentially that
described by Liang and Pardee(1992) (13) and Current Protocols
in Molecular Biology(1994)(24) . Briefly, 5 µg of total RNA
(6- and 24-h samples) was reverse-transcribed (RT) using 15 units of
avian myeloblastosis virus reverse transcriptase (Promega Corp.,
Madison, WI) in the presence of 2.5 µM of an anchored
oligo(dT) primer TAA (5`-TTTTTTTTTTTAA-3`), 8 mM dithiothreitol (Sigma), and 20 µM dNTP (Pharmacia,
Uppsala, Sweden) at 42 °C for 2 h. Samples were then
heat-inactivated at 95 °C for 10 min. PCR was performed using 80 ng
of cDNA from the RT reaction, 2.5 µM T
AA,
1.25 µM of an arbitrarily designed 10-mer, DDMR6
(5`-GACCGCTTGT-3`), 2 µM dNTPs, 1 unit of Taq polymerase (Boehringer Mannheim) and incorporating 1 µCi of
-
S-dATP (Amersham). Of a number of thermostable
polymerases evaluated, Boehringer Taq resulted in reproducible
displays with the least background contamination. The PCR cycling
conditions were: 94 °C for 30 s, 42 °C for 60 s, 72 °C for
30 s, for 40 cycles followed by 5-min elongation time at 72 °C.
Samples were resolved on a 6% (w/v) polyacrylamide gel, the gel dried,
and bands visualized by autoradiography using Kodak AR film (Eastman
Kodak Co.). Bands of interest were excised and placed in 100 µl of
sterilized distilled water, allowed to rehydrate for 10 min, and DNA
eluted from the gel by boiling for 15 min. A 20-µl aliquot was
removed for subsequent amplification by two rounds of the same PCR
reaction conditions but without
-
S-dATP. Enzyme, dNTP
and buffer was re-supplemented prior to the second round of PCR. PCR
products resolved on a 2% (w/v) agarose gel were subsequently extracted
using Qiaex DNA purification kit (Qiagen Inc., Chatsworth, CA), and PCR
products were cloned into pCRScript II (Stratagene, La Jolla, CA). DNA
sequence analysis from both strands (25) was performed using
the Sequenase sequencing kit (U. S. Biochemical Corp.). Sequences were
then compared with sequences in the GenBank(TM) data bank. \begin{rawhtml}
Oligonucleotides specific to the 267 bp sequence of rat SRP54 (Fig. 1B) were synthesized (5`-540F:
5`-CTTGTAGACCCTGAGTTAAAG-3` and 3`-540B: 5`-AGCTGGTCAAAAGCTCCTGCTC-3`)
(shown in Fig. 1B) and subsequently used for
semi-quantitative RT-PCR. A P-labeled internal
oligonucleotide was used to verify PCR products (internal probe:
5`-GGAGTGGTAAAACAACAACGTG-3`) (shown in Fig. 1B).
RT-PCR was performed on 5 µg of total RNA isolated from cells
plated onto plastic or collagen for the times indicated above. For RT,
oligo(dT) (Promega) was used as the primer and the same conditions as
described above with the exception that 1 mM dNTP was
employed. PCR of 80 ng of RT-RNA was performed using 2.5 µM of each primer in the presence of 0.1 mM dNTP.
Amplification of a 415-bp fragment of rat GAPDH was performed to enable
semi-quantitative normalization using oligonucleotides: 5` GAPDH-5
(5`-AACGGATACATTGGGGGTAG-3`) and 3` GAPDH-4
(5`-CATGGAGAAGGCTGGGGCTC-3`), and products were verified with an
internal sense strand oligonucleotide, GAPDH-1
(5`-GCTGTGGGCAAGGTCATCCCC-3`)(26) . Oligonucleotide probes were
end-labeled using T4 polynucleotide kinase (New England Biolabs,
Beverley, CA) incorporating [
-
P]ATP
(Amersham). All oligonucleotides were synthesized using an Applied
Biosystems DNA synthesizer model 381A (Perkin-Elmer, Applied Biosystems
Inc. Division, Foster City, CA). To assess optimal cycle number for
SRP54 primer pairs (540F and 540B), PCR saturation analysis was
performed. Cycle number corresponding to the exponential phase of the
reaction (not shown) was determined to be 25 cycles at 60 °C
annealing temperature. For rat-specific GAPDH primers, optimal product
yield was obtained at 20 cycles at 55 °C annealing temperature.
Figure 1: Differential display gel and sequence identification of rat SRP54. An example of a differential display gel is shown in A. RNA samples were obtained from UMR201 cells grown for 6 or 24 h on plastic (Pl) or type I collagen (Coll), with and without 1 µM RA treatment. The profile of amplified bands was consistent between samples from different experiments and between PCR reactions performed with the same RNA samples. The arrows indicate some of the species up- or down-regulated by the various growth conditions, and the band marked S corresponds to a 267-bp product with homology to murine and canine SRP54. The rat SRP54 nucleotide sequence obtained is shown in B. Nucleotide and amino acid comparisons between rat, mouse, and canine are also shown. The region amplified corresponds to nucleotides 256-522 of canine SRP54 sequence (28) and nucleotides 494-760 of mouse SRP54 sequence(27) . RT-PCR primers are indicated with lines above the sequence (540F(1-22) and 540B(188-167)), and the internal detection oligonucleotide is underlined.
For determination of the half-life of SRP54 mRNA, UMR201 cells were
grown on plastic or collagen for 48 h, then exposed to the inhibitor of
RNA polymerase II, DRB
(5,6-dichloro-1--D-ribofuranosylbenzimadazole; Sigma) at
a concentration of 25 µg/ml. RNA was then extracted from cultures
at timed intervals for up to 24 h.
In order to identify genes potentially regulated by cell-matrix interactions, the technique of dd-PCR was used to compare RNA derived from UMR201 preosteoblastic cells grown on a gel of rat tail type I collagen and compared with RNA derived from cells plated onto tissue culture plastic. Comparison was also made between RNA derived from cells that were either untreated or treated with RA, a known osteoblast differentiating agent(9) . To confirm differentially regulated bands, and to eliminate false positives, dd-PCR was performed at least twice on RNA isolated from experiments conducted months apart. To exclude the possibility of primer or genomic DNA contamination, PCR was performed on non-reverse-transcribed RNA samples and in the absence of template. No PCR products were detected after 40 cycles of the PCR reaction in these controls (not shown).
Many PCR bands appeared differentially regulated between RNA samples from cells that were plated on plastic or collagen and that were either untreated or treated with RA (Fig. 1A). A number of these differentially expressed bands were excised from the sequencing gel, re-amplified, and cloned. Ten bands were subsequently sequenced, two of which were identical, two proved to be smaller fragments of longer sequences, indicating that the 5`-primer could hybridize to multiple sites within the same sequence, and six were unique sequences sharing no homology to sequences in the EMBL or GenBank(TM) data bases. One band of 267 bp (\begin{rawhtml}Fig. 1A) was consistently up-regulated in cells plated onto collagen and was determined to be the rat homolog of the 54-kDa subunit of the signal recognition particle (SRP54). This sequence had a 95 and 94% homology, at the nucleotide level, with mouse (27) and canine (28) SRP54, respectively, with only one amino acid difference in the 86-amino acid sequence (Fig. 1B). Interestingly, the PCR fragment corresponding to the rat homologue of SRP54 resulted from a 5`-primer-5`-primer amplification and not a 5`-primer-3`-primer amplification.
To confirm regulation of SRP54 in response to growth of UMR201 cells on collagen, specific oligonucleotides (540F and 540B) internal to the initial PCR fragment were synthesized corresponding to sequences near the termini of the rat PCR product (see Fig. 1B) and used for semi-quantitative RT-PCR. RNA was extracted at various times after UMR201 cells were plated onto plastic or collagen (Fig. 2A). Fig. 2A shows a Southern blot of the rat SRP54 PCR product verified using a rat-specific internal oligonucleotide as a probe. It is clear that even 1 h after subculturing cells onto collagen, SRP54 mRNA was up-regulated compared with cells on plastic, and this up-regulation was maintained for at least 48 h (not shown). It is of note that at 6 and 24 h, the up-regulation of SRP54 is consistent with that observed by differential display (Fig. 1A). A graphical representation of SRP54 signal normalized to GAPDH is shown in Fig. 2C. The rapid increase in SRP54 mRNA is suggestive of transcriptional activation by collagen. Growth of the UMR201 cells on collagen had no effect on the stability of SRP54 mRNA, which we determined to have an average half-life of 12.4 ± 0.9 h in cells grown on plastic or 14.4 ± 1.4 h in cells grown on collagen (S.E., n = 3). These results support the notion that collagen induces transcriptional activation of SRP54.
Figure 2:
Semi-quantitative RT-PCR of rat SRP54
expression and Northern blot of OP expression in UMR201 cells plated
onto plastic (P) or collagen (C). Semi-quantitative
RT-PCR of SRP54 was performed on samples generated in a time course
experiment where 0 h represents time of subculture. A,
normalization of signals was made with respect to GAPDH. B, OP
was detected using a rat-specific cDNA probe using the same RNA as in
the RT-PCR and comparison made to a GAPDH cDNA probe. C,
quantification of SRP54 mRNA signals to GAPDH mRNA signals and OP mRNA
signals relative to GAPDH mRNA signals was performed by PhosphorImager
analysis: denotes cells grown on plastic, and
denotes
cells grown on collagen. This analysis was performed in two separate
experiments, with similar results.
Since SRP54 is involved in the protein secretory pathway, it was of interest to determine whether up-regulation of a known secreted protein paralleled the increase in SRP54. We have previously shown that osteopontin mRNA was up-regulated in UMR201 cells plated onto collagen for 24 h(7) . We therefore measured OP mRNA levels over the time course period described above for SRP54. The same RNA samples for the experiment of Fig. 2were subjected to Northern blot analysis using a rat osteopontin cDNA probe. Fig. 2B shows that osteopontin mRNA, like that of SRP54, was up-regulated by 1 h after plating cells onto collagen, and this up-regulation was also maintained over the experimental period. A graphical representation of OP mRNA normalized to GAPDH levels is shown in Fig. 2C. Quantification of SRP54 and OP mRNA levels showed that both these species were up-regulated in cells plated onto collagen compared with cells on plastic. SRP54 mRNA remained 2-4-fold higher in cells on collagen compared with cells plated onto plastic, whereas OP mRNA in cells on collagen accumulated over the same period and at 24 h was 6-fold above levels in cells on plastic.
To determine whether the induction of SRP54 mRNA was specific to collagen, UMR201 cells were plated on several non-collagenous matrices containing various cell-binding motifs, including the RGD sequence. In UMR201 cells plated onto fibronectin, laminin, or vitronectin, expression of neither SRP54 nor OP mRNA was regulated differently from cells on plastic (not shown). This suggests that the presence of an RGD motif in the exogenous substrate cannot alone account for the above observations.
The technique of differential display of mRNA, or mRNA fingerprinting, is a powerful tool for comparing the abundance of mRNA species between RNA populations. Here we have shown that this technique was valuable in identifying mRNA species that were regulated in preosteoblastic cells when grown in contact with a physiological substratum. We have previously demonstrated the regulation of gene expression of known osteoblastic markers of differentiation when UMR201 cells were plated on collagen or matrigel, a reconstituted basement membrane preparation(7) .
A number of regulated mRNA species were identified using this procedure, some of which had no corresponding sequence recorded in the EMBL or GenBank(TM) data banks. This may have been the result of amplified sequences being confined mainly to the 3`-untranslated region or they might in fact represent cDNA species for novel mRNA transcripts. One mRNA species was of particular interest, since it was consistently up-regulated in cells on collagen. Sequence analysis identified this mRNA as the rat homologue of SRP54. The sequence obtained was the result of the 5`-primer acting as both sense and antisense primer, without the involvement of the anchored 3`-primer, fortuitously resulting in a sequence of the coding region being obtained.\begin{rawhtml}
Regulation of SRP54 mRNA species has not been reported previously. Although the mRNA species was identified in preosteoblast-like cells, this protein is ubiquitous and has been identified in mammals(27, 28) , yeasts(29, 30) , prokaryotes(27, 28, 31) , and chloroplasts(32) . The regulation of this species may be related to the differentiated state of the cell and its synthetic activity. It is likely that cells actively involved, for example, in organogenesis or repair require up-regulation of components of the synthetic machinery, whereas quiescent cells could down-regulate the expression of these components. Plating of UMR201 cells onto collagen appears to favor a more differentiated state of these cells when compared with cells on plastic(7) . Osteopontin is a known secreted protein of osteoblasts, and the markedly increased expression of this mRNA species may require up-regulation of many components of the protein secretory pathway, including SRP54, to accommodate the throughput of mRNA transcripts of proteins destined for secretion. Thus, cells may require a certain level of SRP54 protein expression to accommodate increased mRNA translation of secreted proteins. This may explain the expression profile found in the present study where SRP54 mRNA expression was rapidly increased, perhaps until a sustainable level of SRP54 protein was attained, followed by reduced steady-state mRNA levels thereafter. The rapid and concordant increase in SRP54 mRNA and OP mRNA after UMR201 cells were plated on to collagen would imply that the matrix evokes downstream signaling pathways to induce transcriptional activation of these genes. The inability of other RGD-containing peptides, such as fibronectin, laminin, or vitronectin, to mimic the induction of mRNA suggests that the presence of an RGD sequence alone is insufficient to elicit such a response. Thus, the collagen-induced activation of these genes may occur via an RGD-independent integrin interaction. It will be intriguing to investigate the signaling pathways that mediate these responses as well as identifying other secreted proteins or other components of the protein secretory pathway where expression is regulated by physiological substrate.
The nucleotide sequence(s) reported in this paper has been submitted to the GenBank(TM) EMBL Data Bank with accession number(s) U29893\begin{rawhtml}[GenBank].