Adenosine (A) to inosine (I) conversion catalyzed by adenosine deaminases acting on RNA (ADAR) is an evolutionally conserved process, occurring in organisms from unicellular protozoa to humans 12. Through site-specific modification of pre-mRNAs, this process provides an important post-transcriptional mechanism for expanding the functional diversities of RNA and protein products, such as those that encode the glutamate receptors and serotonin receptors 34. In contrast, nonspecific editing is more frequent and has been considered mainly implicated in host defense mechanisms 5.

Due to the use of different promoters, human ADAR1 has two major variants: The full-length form p150 is expressed from an interferon (IFN) -inducible promoter and predominantly localizes to cytoplasm. Use of a constitutive promoter, in contrast, produces an N-terminally truncated, predominantly if not exclusively nuclear p110 protein that is not induced by IFN 67. Owing to its special cytoplasmic location and elevated deaminating activity during infection, IFN-inducible p150 is believed to play a role in antiviral defense against viruses that replicate in the cytoplasm 89.

The physiological importance of ADAR1 has been confirmed by phenotypic analysis of null mutants in previous studies. Inactivation of ADAR1 gene has been reported to cause lethality in ADAR1^+/- chimeric mice and ADAR1^-/- embryos, along with severe impairment of liver structure and reduced hepatocyte cell density 101112. The remarkable observation that among many ADAR1 deleted embryonic tissues that underwent apoptosis, the highest level of apoptosis was within the liver and regions exhibiting excessive apoptosis in ADAR1^-/- embryos corresponded to tissues expressing the highest levels of ADAR1 in wild-type embryos indicated an essential role of ADAR1 in the normal development of non nervous tissues 10. Moreover, compared with wild-type MEF (mouse embryonic fibroblasts) cells, ADAR1^-/- MEF cells were prone to apoptosis when subjected to serum deprivation, and expression of ADAR1 p150 increased significantly in wild-type MEF cells during serum deprivation 12, perhaps indicating a special requirement of ADAR1 p150 for cell survival.

Recently, Samuel and his colleagues reported that small amount of ADAR1 p150 could be detected in almost all tissues of healthy adult mice 13. Expression of p150 was found to be least abundant in brain tissue of normal mice, and this seems somewhat correlated with the previous observation that no abnormality was detected in ADAR1-deleted embryonic brain 101112. They also found that p150 is most abundant in liver of mice infected with Salmonella and where it is also the major form of ADAR1. Taken together, these data suggest that endogenous ADAR1 p150 protein may play a critical role in the normal development and maintenance of bodily tissues, especially for liver. However, despite the ubiquitous expression of ADAR1 and the correlated large amount of I-containing mRNA (I-mRNA) throughout the body 11415, as of yet, only a few genes with editing sites in coding regions have been identified as endogenous substrates of ADAR1 3416.

The expression and regulation of ADAR1 p150 in human tissues has not been fully characterized thus far. In HeLa cells, the simultaneous presence of two forms of ADAR1 has been confirmed by both Western-blotting and immunofluorescence analysis 1718. In the present study, by using a method based on hammerhead ribozyme technique, we specifically knocked down the expression of mRNA for p150 ADAR1 isoform in HeLa cells and first revealed that endogenous p150 is necessary for the proper control of cell proliferation.

HeLa Tet-On cells transfected with the constructed pTRE-ADAR1-RZ or the control carrier were named as HeLa-Rz and HeLa-P cell clones, respectively. A total of 24 HeLa-Rz cell clones were collected and measured for Dox-induced alteration in expression of mRNA of p150 ADAR1. The relative abundance of ADAR1 p150 was similar for all cell clones in the absence of Dox (data not shown). Addition of 2 μg/ml of Dox significantly reduced the level of mRNA of p150 ADAR1 isoform in a few HeLa-Rz cell clones, and the inhibitory effect was in a time-dependent manner (Fig. 1). The result of Western blotting analysis was shown in Fig. 2: p150 isoform of ADAR1 was detected in both HeLa-Rz cells and HeLa-P cells by the antibody we used. After Dox treatment, the amount of p150 protein was decreased significantly in HeLa-Rz cells, in contrast, expression of p150 in HeLa-p cells was nearly not affected.

To reveal the potential correlations between level of p150 ADAR1 isoform and cellular biological properties, we examined cell viability of different HeLa-Rz cell clones in response to Dox treatment. The results showed that, in addition to the decrease of p150 expression, relative cell viability of HeLa-Rz clones was also reduced (with an inhibitory rate in the range of 25% to 38.0%) by three days of Dox induction, whereas the viability of HeLa-p cells was not affected by Dox treatment (Fig. 3A). A Dox-induced downward shift in the cellular growth curve was observed in a HeLa-Rz cell clone (shown in Fig. 3B). The calculated population doubling time (Gt) (21.52 ± 1.20 h) of HeLa-Rz cells was prolonged (32.43 ± 3.40 h, P < 0.01) significantly by Dox treatment. However we did not observed obvious morphological changes under the light microscope.

HeLa-Rz cells were grown in medium containing 2 μg/mL Dox for 48 h, causing the expression level of ADAR1 mRNA to decrease. Flow cytometry analysis detected a constant increase in G₁ DNA content (from 38.87 ± 0.11 % to 46.53 ± 0.10 %, p < 0.05) in comparison with the control group. The percentage of cell DNA in replication phase S slightly decreased, but statically the change was not significant (39.94 ± 0.08 % vs 37.49 ± 0.07 %, p > 0.05). These data suggest that Dox treatment, acting through knockdown of the p150 ADAR1 mRNA, could lead to an arrest of cells in G₁ phase, a delayed transition into S phase, and eventually restrained proliferation of cells (Fig 4). Under our experimental condition, Dox did not induce apoptosis.

A single HeLa-Rz cell clone was picked out based on its high sensitivity to Dox induction and the cells were cultured. Nude mice were given subcutaneous injections of cultured HeLa-Rz cells and the growth rate of cell transplants was monitored. At 5 days post inoculation, all animals developed a palpable tumor at the injection site, indicating the cell tumorigenecity was not altered. However the rate of tumor growth in the Dox-treated group was significantly slower compared with the control group (Fig. 5). This difference became detectable (P < 0.05) by day 11. By day 23 the mean tumor size in Dox-treated mice was 1.38 ± 0.34 cm³, whereas in the control group it had reached 2.60 ± 0.69 cm³, which corresponding to an about 60 % inhibitory rate of tumor growth. The health of the mice was not affected as evaluated by the lack of body weight loss. Taken together, these data indicate that decrease of p150 ADAR1 isoform significantly inhibited growth of transplanted HeLa-Rz cells, but does not affect tumor induction in nude mice.

The sequences of ADAR1 from human, rat, and mouse are highly conserved, all having a unique N-terminus (containing two tandemly arranged Z-DNA-binding domains), three double-stranded RNA-binding domains (dsRBDs) and a conserved deaminase domain at the C-terminus 6. Its distinct structural architecture, tightly regulated expression and intracellular distribution set ADAR1 apart from other known ADAR gene family members, ADAR2 and ADAR3 222324. Furthermore, the discrepancy between its widespread expression within the body and the few known substrates indicates that in vivo function of ADAR1 may not be restricted to nuclear pre-mRNA editing 131516.

Due to its interferon-inducible expression and its predominantly cytoplasmic localization, p150 isoform of ADAR1 has been considered involved in host defense mechanisms against viruses that replicate in the cytoplasm 89. More recently, the observation that serum deprivation significantly increased cytoplasmic level of p150 expression in MEF cells suggests that p150 might also play a role critical for the promotion of cell survival 11.

In the present study, by using RT-PCR and Western blotting methods, we demonstrated that endogenous p150 isoform (full-length isoform of human ADAR1) of ADAR1 is expressed abundantly in HeLa cells. In order to study its biological function, we specifically down regulated the level of mRNA for p150 protein by using a hammerhead ribozyme-based technique. Our results revealed that a several fold knockdown of ADAR1 p150 inhibited cell proliferation (by a maximum inhibitory rate of 38%) significantly. In addition, cell cycle progression of p150 suppressed cells was characterized by an excessive retention of cells in G₁ phase and delayed transition into S phase. However, we did not find any obvious cellular morphological changes under the light microscope. In nude mice, the growth rate of transplanted HeLa cells was also significantly reduced by down-regulation of ADAR1 p150 expression.

The molecular mechanisms underlying the action of p150 ADAR1 protein to maintain cellular proliferation is still under investigation. In vitro, the enzyme can act on almost any double stranded substrate of sufficient length, showing little site selectivity 25. Secondly, because any RNA that is at least partially double-stranded represents a potential substrate for A-to-I editing, ADAR1 may interfere with other cellular processes that rely on dsRNA molecules, such as RNAi 26 and NF90 proteins (including NF110, NF90 and NF45) 23. Finally, supported by the observation that both expression and activity of ADAR1 p150 are elevated in lymphocytes in response to inflammation 27, it appears that cytoplasmic editing activity of ADAR1 p150 might also be involved in the regulation of gene expression under special pathological conditions.

Based on our study, endogenous expression of ADAR1 p150 protein is necessary for the proper control of cell growth. p150 protein is also capable of responding to "unfavorable stimulations" and thus involved in host defense mechanisms through its inducible expression, cytoplasmic accumulation and shuttling activity between the nuclear and cytoplasmic compartments 691722. Recent bioinformatics analysis has revealed that A-to-I editing modification occurs in at least 30 different organs with different frequencies and most editing events are found within Alu elements embedded in the non-coding regions of human transcriptome, which is suggested to be engaged in the modulation of tumor cell growth and differentiation 2829303132. Further investigation is required to address the questions whether and which form of ADAR1 is associated with tumor development.

Our results suggest that normal expression and functioning of p150 ADAR1 isoform is essential for the maintenance of proper cell growth. The mechanisms underlying the action of ADAR1 p150 might include both cytoplasmic editing of currently unknown dsRNAs and interacting with other cellular dsRNA-related processes.

The author(s) declare that they have no competing interests.

HW participated in the design of the study, performed plasmid construction, cell culture, cell transfection and RT-PCR analysis, and drafted the manuscript, ZH performed Western blotting analysis, YW and XM participated in the animal experiment and performed statistical analysis. XL conceived of the study, participated in its design and coordination and revised the article critically for important intellectual content. All authors read and approved the final manuscript.