Department of Molecular Cell Biology, Laboratory for Cytochemistry and Cytometry, Leiden University Medical Center, Wassenaarseweg 72, 2333 AL Leiden, The Netherlands
Corresponding author (e-mail: R.W.Dirks{at}lumc.nl)
Accepted October 12, 2001
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SUMMARY |
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Key words: Fluorescent in situ hybridization, Confocal scanning laser microscopy, RNA polymerase II, Human cytomegalovirus
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Introduction |
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At least two mechanisms indirectly link mRNA synthesis to the transport of mature mRNAs to the cytoplasm. Both of these function through the splicing reaction and determine whether a transcript can access the nuclear export pathways of the cell. One mechanism involves splicing commitment factors (organized in spliceosomes), which actively retain intron-containing pre-mRNAs in the nucleus until the splicing process removes the remaining introns and thereby the splicing commitment factors (Chang and Sharp, 1989; Legrain and Rosbash, 1989
). This step may be rate limiting in some instances. In addition, export of mRNA that is defective in splicing or 3' end processing and synthesized from mutated expression constructs is blocked at this step (Custodio et al., 1999
; Johnson et al., 2000
). The second mechanism concerns the selective recruitment of specific export factors, such as the TAP protein (Grüter et al., 1998
), to fully processed mRNAs (Luo and Reed, 1999
). This protein contains an essential domain that functions both as a nuclear export signal and as a binding domain for components of the nuclear pores (Görlich et al., 1999
; Kang and Cullen, 1999
; Katahira et al., 1999
).
These intimate relationships between RNA synthesis, RNA processing and RNA transport are also reflected in the spatial-temporal organization of the genes and factors involved in these processes. Nascent transcripts are confined to several thousand nucleoplasmic sites or transcription factories (Fay et al., 1997) (reviewed in Jackson et al., 2000
). Each factory contains
30 active polymerases with their associated transcripts (Jackson et al., 1998
). Efficient processing of these transcripts requires the recruitment of splicing factors such as SF2/ASF to sites of active genes in vivo (Misteli et al., 1997
; Misteli and Spector, 1999
; Eils et al., 2000
). It has been proposed that a large number of these components pre-assemble into a transcription/processing complex, followed by the recruitment or transport of this complex to the active genes (Gall et al., 1999
). The large subunit of the elongating form of PolII and several splicing factors are present in numerous nuclear domains or speckles at the light microscope resolution level in addition to a diffuse nucleoplasmic staining (Spector, 1993
; Bregman et al., 1995
; Mortillaro et al., 1996
; Zeng et al., 1997). Moreover, the activity and localization of splicing factors is determined by their phosphorylation state (Misteli and Spector, 1998
).
When a particular gene is transcribed at a high level, new transcripts may accumulate at or near the transcription site in foci that have an elongated dot or track-like appearance. This has been shown for endogenous genes such as human collagen 11 and ß-actin (Xing et al., 1995
; Femino et al., 1998
) and for integrated viral genes (Lawrence et al., 1989
; Dirks et al., 1997
). In these cases, the active gene is often localized at one extreme of an elongated dot. This suggests that the majority of mRNAs in the elongated dot are detached from the gene. Although the majority of RNA processing is supposed to occur cotranscriptionally, elongated dots may represent sites in which pre-mRNA processing is completed or may represent an early stage of RNA export (Dirks et al., 1997
; Johnson et al., 2000
; Melcák et al., 2000
). In rat 9G cells, which we use in this study, it has been demonstrated that nuclear foci contain HCMV IE RNA exon and intron sequences as well as splicing factors. The splicing reaction is therefore thought to continue within the elongated dot-like structures (Raap et al., 1991
; Dirks et al., 1997
; Snaar et al., 1999
).
In this study, we use a quantitative method based on fluorescent in situ hybridization (FISH) in combination with confocal scanning laser microscopy (CSLM) to investigate the spatial and temporal relationships of HCMV IE mRNA synthesis and nuclear export in response to inactivation and activation of PolII. On the basis of these measurements we show that nuclear HCMV IE transcripts represent two subpopulations with distinct kinetic behavior, namely those in nuclear foci (at or near the transcription site) and those dispersed throughout the nucleoplasm.
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Materials and Methods |
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Cell fixation and in situ hybridization
Cells were fixed and permeabilized as described (Dirks et al., 1993). Briefly, rat 9G cells were washed in PBS for 10 seconds and fixed with 3.7% formaldehyde (Merck, Darmstadt, Germany) containing 5% acetic acid in PBS for 15 minutes at room temperature. Cells were subsequently washed twice in PBS and stored in 70% ethanol at 4°C. Prior to hybridization, cells were washed in deionized water and pretreated with 0.1% pepsin (Sigma) in 0.01 M HCL for 30 seconds at 37°C. Cells were then washed in deionized water, dehydrated in a graded ethanol series and air-dried to prevent uncontrolled dilution of probes. Detection of HCMV-IE mRNA by DNA probes was carried out with plasmid pSS containing the 5.0 kb SphI-SalI genomic fragment of the immediate-early region (Boom et al., 1986
). Probes for intron 1 and exon 4 sequences were generated by PCR from plasmid pSS with specific primers. Probes were labeled with digoxigenin-, biotin- or FITC-dUTP by nick translation (Roche Diagnostics GmbH, Mannheim, Germany) and purified over PCR purification columns according to instructions provided by the manufacturer (Qiagen, Venlo, the Netherlands). Probes were dissolved in 60% deionised formamide, 2xSSC (0.3 M NaCl, 0.03 M Na-citrate), 10 mM EDTA, 25 mM NaH2PO4 pH 7.4, 10% dextran sulfate and 250 ng/µl sheared herring sperm DNA at a final concentration of 5 ng/µl. Glass slides containing rat 9G cells were fixed, pretreated with pepsin and hybridized with a probe as described previously (Dirks et al., 1993
). Probe and target sequences were denatured simultaneously by placing the slides on an 80°C metal plate for two minutes. Hybridizations were performed at 37°C overnight in a moist chamber.
Previously, we have shown that the hybridization patterns obtained by this procedure were very similar to those obtained when cells are submitted to a much stronger fixation procedure and examined by electron microscopy (Macville et al., 1995).
Post-hybridization washes and immunofluorescence
Cells were washed three times in 60% formamide, 2xSSC for 10 minutes each at 37°C and two times five minutes in Tris-buffered saline (TBS: 150 mM NaCl, 100 mM Tris-CL pH 7.4) containing 0.05% Tween 20 (Biorad, Hercules, California, USA) at room temperature. Digoxygenin-labeled probes were detected by anti-digoxin monoclonal antibody (Sigma Aldrich, St. Louis, MA, USA; dilution 1:1000) followed by goat anti-mouse Alexa594 (Molecular Probes Inc. Eugene, OR; dilution 1:500). Probes labeled with biotin were detected by Streptavidine-Alexa594 (Molecular Probes Inc. Eugene, OR, USA; dilution 1:400). All antibodies were diluted in TNB (TBS containing 0.5% (w/v) blocking reagent (Roche Diagnostics GmbH, Mannheim, Germany)) and incubated for 45 minutes at 37°C. Cells were dehydrated through a graded ethanol series and mounted in Vectashield (Vector Laboratories, Inc., Burlingame, California, USA) containing 50 µg/ml 4',6'-diamidino-2-phenyl indole (DAPI) as a DNA counterstain.
Microscopy and quantification of fluorescence by confocal scanning laser microscopy
Fluorescence microscopy was carried out with a Leica DM epifluorescence microscope equipped with a 100 W mercury arc lamp and appropriate filter sets. Digital images were captured with a cooled CCD camera (Photometrics, Tucson, Arizona, USA) and processed using SCIL-image (Multihouse, Amsterdam, the Netherlands) and Adobe Photoshop. Confocal images were recorded on a Leica TCS confocal scanning laser microscope (CSLM) (Leica Microsystems, Heidelberg, Germany) equipped with a 100xPL APO NA 1.4 Leica objective and an Argon/Krypton laser at an excitation wavelength of 567 nm. Image stacks of expressing and non-expressing cells in the same visual field were collected for quantitative analysis of the integrated fluorescence intensity in accumulations of HCMV IE transcripts (nuclear foci) and in the remainder of the nucleus in such a manner that saturation of the recorder (photomultiplyer tube) did not take place. The laser intensity and scanning speed were kept constant to avoid the interference of different levels of photobleaching during the measurements. The integrated fluorescence intensity in specified regions (of known area) of the nucleus was calculated in three-dimensional representations of the nucleus on the basis of the collected image stacks, which is a feature included in the Leica TCS NT software package. Additional calculations were carried out in Microsoft Excel. The integrated fluorescence intensity in the HCMV DNA integration site in non-induced cells was used as a reference, as all cells contain the same integrated tandem repeat of HCMV genes. All values were averaged over five to 10 cells. These cells were randomly chosen from the pool of HCMV IE expressing cells. Differential interference contrast images were also recorded for each cell to provide information about intracellular structures.
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Results |
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After inhibition of PolII, HCMV IE transcripts exit more rapidly from nuclear foci than from the diffuse nucleoplasmic pool
As integrated fluorescence intensity in the nuclear RNA foci decreased approximately threefold within 10 minutes of inhibition of PolII activity, the half time of this process is approximately two minutes (Fig. 1A; Table 1). The ratio of transcribed intron 1 sequences and transcribed total HCMV-IE sequences remained constant throughout the foci at all time-points (data not shown). This suggests that the release of transcripts from the RNA foci correlated with the completion of the splicing reaction (Dirks and Raap, 1995; Snaar et al., 1999
). After
30 minutes, the level of fluorescence in the track was comparable to that in the integration site, indicating that no or only a few transcripts are present at the transcription site. The integrated fluorescence intensity of the dispersed nuclear transcripts decreased with much slower rates (Fig. 1B; Table 1) after PolII inactivation (half time of
10 min). After
120 minutes, the nuclei of these cells reached an integrated fluorescence intensity closely resembling that of HCMV-IE negative cells. The inhibitory mechanism of PolII did not seem to influence the kinetics of these processes, as the integrated fluorescent intensity decreased with similar kinetics whether PolII was inhibited by AMD or by DRB (Table 1).
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Discussion |
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The kinetics of HCMV IE activation in rat 9G cells are in agreement with the kinetics of ß-actin gene activation in rat kidney cells (Femino et al., 1998). In both cell types, the number of transcripts at the transcription site increases in a linear fashion during the first five minutes of gene activation. At this time, transcripts become visible in nuclear RNA foci or elongated dots. Mature mRNAs are detected in our system at nuclear sites distinct from, but surrounding, the nuclear RNA foci from five minutes onwards. This implies that both transcription and pre-mRNA processing of the newly transcribed
6 kb HCMV IE messengers can be completed within five minutes. Comparison with the reported rates of PolII transcription, which are 1.7-2.5 kb/min for human PolII (Tennyson et al., 1995
) and
1.1-1.4 kb/min for rat PolII (Femino et al., 1998
), suggests that most or all of this time will be required for mRNA transcription. Pre-mRNA processing must therefore be mostly cotranscriptional in these early phases of transcription.
Inactivation of RNA PolII by DRB or AMD results in the disappearance of accumulated HCMV IE transcripts with a calculated half time of approximately two minutes. Melcák et al. (Melcák et al., 2000) observed a similar reduction in the amount of Epstein-barr virus mRNA, as judged qualitatively by the length of the elongated dots that accumulated at transcription sites in Namalwa cells after DRB or AMD inhibition. As efficient release of transcripts from the spliceosome requires the completion of pre-mRNA processing (Custodio et al., 1999
), the decrease in the rate of integrated fluorescence intensity appears to mirror the rate at which the remaining introns are removed from the accumulated transcripts. Several protein factors may be involved in this transient immobilization of transcripts at and near the transcription site. It may involve splicing commitment factors, but it may also be a function of RNA PolII, which remains present in a complex with splicing factors after termination of transcription (Snaar et al., 1999
). The subsequent release of spliced transcripts from spliceosomes may involve putative RNA helicases (Company et al., 1991
; Ohno and Shimura, 1996
; Schwer and Meszaros, 2000
) and the small GTPase Ran (Grimm et al., 1997
). Concomitant with RNA synthesis and processing, the cap-binding proteins, the poly(A)-binding protein PABP2 and various other mRNA-binding proteins associate with mRNAs to mediate their transport (Visa et al., 1996
; Calado et al., 2000
; Huang and Steitz, 2001
; Le Hir et al., 2001
; Lei et al., 2001
). The capacity of these processes may also be exceeded by the transcription rate of the HCMV IE gene, possibly resulting in the saturation of the entire transport system. Interestingly, yeast strains carrying mutations in mRNA nuclear export factors were shown to accumulate mature mRNAs in foci that coincide with sites of transcription (Jensen et al., 2001
).
Monitoring the decrease in nuclear fluorescence after treatment of rat 9G cells with DRB revealed that HCMV-IE mRNA export takes place with a half time of 10 minutes. Previously, mRNA export from oocyte nuclei had been reported with half times of 2.4 minutes (Dargemont and Kühn, 1992
) and 30 minutes (Jarmolowski et al., 1994
). The half-time value measured in this study is consistent with the value measured by Jarmolowski et al. (Jarmolowski et al., 1994
), considering the fact that the diameter of an oocyte nucleus is at least five times larger than the diameter of a rat fibroblast nucleus. Differences in transport rates may also be caused by discrepancies in the nuclear complexity and the compactness in these cell types. Transport of in vitro transcribed mRNA in oocyte nuclei was analyzed upon microinjection. Interestingly, Jarmolowski et al. (Jarmolowski et al., 1994
) measured a lag time of 20-25 minutes before export of mRNA. It is likely that this period was needed to assemble a transport-competent complex. Apparently, the formation of such a complex is much more efficient when coupled to transcription, as HCMV-IE transcripts are exported from the gene within five minutes of the initiation of transcription. This is also consistent with data presented by Pallavicini et al. (Pallavicini et al., 1994
), who studied c-myc expression under control of a heat shock promoter in CHO-like cells. Upon heat shock, c-myc transcripts started to accumulate in cell nuclei within 10 minutes and remained there, but after returning the cells to 37°C it took them one hour to be transported to cytoplasm. This suggests that either splicing or the formation of transport-competent complexes does not occur during heat shock.
As previously described, HCMV-IE transcripts radiate in all directions upon release from the transcription site and are eventually present throughout the nucleoplasm in a punctate pattern (Dirks and Raap, 1995; Macville et al., 1996
). Transcripts are detected at increasing distances from the transcription site at increasing transcription times and throughout the nucleoplasm after approximately 30 minutes. A diffusion rate of
0.13 µm2/sec is calculated for this process. Much faster rates of RNA transport have been reported by Politz et al. (Politz et al., 1999
) using hybridizing oligo (dT) labeled with chemically masked fluorescein to nuclear poly(A) RNA followed by spot photolysis and recording the distribution of fluorescence. After uncaging fluorescein, fluorescence spread within 30 seconds in all directions throughout the nucleus at a calculated diffusion rate of 0.6 µm2/sec. It was therefore concluded that mRNA export is a process of free diffusion, which does not require energy. It should be noted, however, that there exist many different types of poly(A) RNA in the cell nucleus that are poorly characterized. For example, it is still not known what type of poly(A) RNA is present in speckle domains containing splicing factors and other processing and transcription factors. Earlier, Politz et al. (Politz et al., 1998
) measured a broader range of diffusion rates by fluorescence correlation microscopy, suggesting that different pools of poly(A) RNA that do not all necessarily leave the cell nucleus but may move at fast speed may indeed exist. The mRNAs in transit to the cytoplasm may move at a much slower speed because they are packed in an RNP particle (Singh et al., 1999
). Miralles et al. (Miralles et al., 2000
) demonstrated that Balbiani Ring RNP particles do not always diffuse freely through the nucleoplasm. Instead, they have been observed to interact with fibers of specific structure and composition (Miralles et al., 2000
). Notably, poly(A) RNA was shown to move in nuclei at a rate consistent with free diffusion but they did not accumulate in the cytoplasm. We observed that fluorochrome-labeled poly (dT) hybridized to poly (A) RNA in living cells was poorly exported towards the cytoplasm, indicating that hybridized mRNAs may escape from the regular transport mechanism (C. Molenaar, H.J.T. and R.W.D., unpublished).
Furthermore, our results and those of others indicate that mRNA export is at some stage energy dependent because transport is blocked when cells are incubated at 4°C or at slightly lower temperature (Dargemont and Kühn, 1992; Jarmalowski et al., 1994
; Melcák et al., 2001
). Consistent with these observations, Calado et al. (Calado et al., 2000
) reported that no transport of PABP2 to the cytoplasm takes place at 4°C. Another argument opposing a free diffusion model of RNA export is the presence of nucleoplasmic structures that at some stage mediate RNA export by transient interactions [for example see Strambio-de-Castillia et al. (Strambio-de-Castillia et al., 1999
)]. In conclusion, this study demonstrates that levels of transcription, pre-mRNA processing and transport of HCMV IE mRNA are rapidly regulated in response to inhibition or activation of PolII. These processes are tightly linked in time and space. Furthermore, our results indicate that nucleocytoplasmic transport of these transcripts may occur in an energy-dependent active process.
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ACKNOWLEDGMENTS |
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