Patent Description:
Double-stranded RNA (dsRNA), first discovered in retroviruses, has been considered as a byproduct of viral replication in mammals. The dsRNA expressed in mammalian cells is recognized by innate immune response proteins to induce interferons, inhibit protein translation and induce apoptosis. The interesting thing in the dsRNA-mediated signal transduction is that the immune response protein recognizes a specific structure of RNA, such as the secondary structure rather than the specific sequence.

Although dsRNA is closely related to immune response through the antiviral signal transduction, evidences have been reported that human cells naturally express dsRNA capable of regulating antiviral machinery in various cellular environments. RNA in the mitochondria can exist as intermolecular dsRNA, which can bind to PKR and regulate the signaling activity thereof. It has also been found that the accumulation of endogenously encoded dsRNA is associated with the development of autoimmunity and age-related macular degeneration (<NPL>).

The patent application <CIT> discloses senescence markers which are ds micro RNA for breast cancer and their expression level as marker for the disease as well as for the reponsisiveness to a treatment. This patent application discloses also a method for evaluating a senescencece inhibitor and cancer inhibitor comprising as an effective component a agenetranscript of the senescence marker.

The international patent application <CIT> discloses the use of dsRNA as diagnostic markers for Sjögren's syndrome or arthritis.

The publication of <NPL>) suggests to use Spirropyran for labelling dsRNA.

The publication of <NPL>) discloses the expression level of micro RNAs (mi RNAs) that are single stranded endogeneous non coding small RNAS from <NUM> to <NUM> nucleotides in autoimmune diseases.

The present inventors confirmed that the merocyanine compound can be effectively used for detecting dsRNA and comparing the expression levels between samples, and that the disease related to dsRNA overexpression can be diagnosed by measuring the expression level of dsRNA, thereby completed the present invention.

It is an object of the present invention to provide a composition for detecting dsRNA comprising a merocyanine compound, a salt thereof or an isomer thereof.

Disclosed but not part of the claimed invention is a kit for detecting dsRNA comprising the composition of the present invention.

Disclosed but not part of the claimed invention is a method for detecting dsRNA using the merocyanine compound of the present invention.

Disclosed but not part of the claimed invention is method for providing information for the diagnosis of cancer.

It is another object of the present invention to provide a method for predicting the responsiveness of a cancer patient to an anticancer agent.

Disclosed but not part of the claimed invention is a method for providing information for the diagnosis of degenerative joint disease.

Disclosed but not part of the claimed invention is a method for providing information for the diagnosis of Sjogren's syndrome.

To achieve the above objects, the present invention provides a composition for detecting dsRNA comprising a merocyanine compound represented by formula <NUM> below, a salt thereof or an isomer thereof:
<CHM>
(In formula <NUM>, R is - CH<NUM>CH<NUM>CH<NUM>N+ (CH<NUM>) <NUM>).

Disclosed but not part of the claimed invention is a method for detecting dsRNA comprising the following steps:.

Disclosed but not part of the claimed invention is a method for providing information for the diagnosis of cancer comprising the following steps:.

The present invention also provides a method for predicting the responsiveness of a cancer patient to an anticancer agent comprising the following steps:.

Disclosed but not part of the claimed invention is a method for providing information for the diagnosis of degenerative joint disease comprising the following steps:.

Disclosed but not part of the claimed invention is a method for providing information for the diagnosis of Sjogren's syndrome comprising the following steps:.

The merocyanine compound of the present invention causes a spectral change of a hypochromic shift in the vicinity of the wavelength of <NUM> by intercalation between dsRNA nucleotide pairs, and the spectral change shows high accuracy and reproducibility, so the merocyanine compound of the present invention can be effectively used for detecting dsRNA and comparing the expression levels between samples.

In addition, the present invention can provide information for the diagnosis of degenerative joint disease or Sjogren's syndrome, as well as cancer by measuring the expression level of dsRNA separated from a sample of a test subject and comparing it with that of the normal control group. Further, the responsiveness of a patient to the treated drug can be predicted by treating the sample with a drug and measuring the expression level of dsRNA.

Disclosed but not part of the claimed invention is a composition for detecting dsRNA comprising a merocyanine compound represented by formula <NUM> below, a salt thereof or an isomer thereof:
<CHM>
(In formula <NUM>, R is -CH<NUM>CH<NUM>CH<NUM>N+(CH<NUM>)<NUM>).

The merocyanine compound can be an isomer produced by irradiating UV to a spiropyran compound represented by formula <NUM> below:
<CHM>
(In formula <NUM>, R is - CH<NUM>CH<NUM>CH<NUM>N+(CH<NUM>)<NUM>).

When the spiropyran compound is exposed to ultraviolet light, the carbon-oxygen bond inside is decomposed and the three-dimensional structure is changed to be isomerized to the merocyanine compound. Since the isomerization between the spiropyran and the merocyanine is reversible, when the visible light is irradiated to the merocyanine compound, it can be isomerized again to the spiropyran compound.

The merocyanine compound can be intercalated between dsRNA nucleotides. As the merocyanine compound is intercalated between dsRNA nucleotides, the merocyanine compound is protonated and can cause changes in UV-Vis absorbance spectrum. Particularly, as the merocyanine compound is intercalated between dsRNA nucleotides, spectral changes of hypochromic shift can appear at the wavelength of <NUM>.

The kit can additionally include an UV-Vis spectrometer. In addition, the kit can additionally include a single strand RNA degradation enzyme, a solvent (buffer), and other reagents.

The solvent can be phosphate buffer, carbonate buffer, or cacodylate buffer. Also, the solvent may or may not contain ions. Specifically, the solvent may not contain ions.

The single strand RNA degradation enzyme can be RNase T1 or RNase I, specifically, RNase T1, but not always limited thereto.

In a preferred embodiment, the present inventors irradiated UV to the synthesized spiropyran to produce merocyanine, an isomer of spiropyran. As a result, it was confirmed that spiropyran was not combined with dsRNA, so no change was observed in the UV-Vis absorbance spectrum, whereas merocyanine was intercalated with dsRNA to change the absorbance spectrum of merocyanine (see <FIG>).

It was also confirmed that merocyanine interacted more strongly with poly GC than poly AU, and more strongly with dsRNA in a solution without ions than a solution with ions (see <FIG>).

It was confirmed that the red merocyanine was changed to colorless merocyanine as the dsRNA of poly GC was intercalated with merocyanine (see <FIG>).

It was confirmed that merocyanine did not bind to single nucleotide nucleic acid and was effective in detecting dsRNA of <NUM> bp or more (see <FIG> and <FIG>).

It was also confirmed that the higher the concentration of dsRNA, the higher the rate of change in absorbance of merocyanine. And it was confirmed that the amount of dsRNA between samples could be compared by quantifying the change in absorbance of merocyanine (see <FIG>).

It was also confirmed that merocyanine was intercalated not only with synthetic dsRNA, but also with dsRNA extracted from real cells (see <FIG>).

The merocyanine compound causes a spectral change of a hypochromic shift in the vicinity of the wavelength of <NUM> by intercalation between dsRNA nucleotide pairs. And the amount of dsRNA between samples can be compared by quantifying the change in absorbance of merocyanine. The spectral change shows high accuracy and reproducibility, so the merocyanine compound of the present invention can be effectively used for detecting dsRNA and comparing the expression levels between samples.

(In formula <NUM> and formula <NUM>, R is - CH<NUM>CH<NUM>CH<NUM>N+(CH<NUM>)<NUM>).

In the above method, the RNase of step <NUM>) can be RNase T1, but not always limited thereto, and an enzyme capable of degrading single strand RNA can be used without limitation. The RNase T1 can degrade single strand RNA (ssRNA) and hairpin loops.

The reaction of step <NUM>) can be performed in a solution with or without ions. Specifically, the reaction of step <NUM>) can be performed in a solution without ions, and the merocyanine compound exhibits a positive charge, so that the ions in the solution can interrupt the intercalation of the merocyanine compound with dsRNA.

The amount of dsRNA in step <NUM>) can be measured by UV-Vis spectroscopy, and specifically, the amount of dsRNA in step <NUM>) can be measured by the change in absorbance at the wavelength of <NUM>. As the merocyanine compound is intercalated between dsRNA nucleotides, the merocyanine compound is protonated and can cause changes in the UV-Vis absorbance spectrum. Particularly, as the merocyanine compound is intercalated between dsRNA nucleotides, spectral changes of hypochromic shift can occur at the wavelength of <NUM>.

The sample of step <NUM>) can be any one selected from the group consisting of blood, serum, plasma, body fluid, saliva, urine, cells and tissues, but not always limited thereto.

The measurement of the expression level of dsRNA in step <NUM>) can be performed by RT-PCR or UV-Vis spectroscopy, but not always limited thereto. Particularly, the expression level of dsRNA can be measured by extracting total RNA from a sample of a test subject, synthesizing cDNA, and then performing RT-PCR with a primer capable of amplifying dsRNA. Or, the measurement can be performed by extracting total RNA from a sample of a test subject, and measuring the absorbance changes that appear in response to the merocyanine compound. Specifically, the measurement of the expression level of dsRNA in step <NUM>) can include the following steps:.

The RNase of step ii) can be RNase T1, but not always limited thereto, and an enzyme capable of degrading ssRNA can be used without limitation. The said RNase T1 can degrade ssRNA and hairpin loops.

The reaction of step iii) can be performed in a solution with or without ions. Specifically, the reaction of step iii) can be performed in a solution without ions, and the merocyanine compound exhibits a positive charge, so that the ions in the solution can interrupt the intercalation of the merocyanine compound with dsRNA.

The absorbance of step iv) can be measured at the wavelength of <NUM>.

In addition, the measurement of the expression of dsRNA can further include a step of calculating the rate of change in absorbance by comparing the absorbance of step iv) with that of the reaction solution without dsRNA. Cancer cells and normal cells can be distinguished according to the calculated rate of change in absorbance. According to an embodiment of the present invention, the expression level of dsRNA in cancer cells can be higher than the expression level of dsRNA in normal cells.

In a preferred embodiment, the present inventors treated the merocyanine compound to each dsRNA extracted from normal cells and cancer cells, and measured the rate of change in absorbance at <NUM>. As a result, the rate of change in dsRNA absorbance in cancer cells was higher than that in normal cells, which confirmed that the expression level of dsRNA in cancer cells was higher than that in normal cells (see <FIG>).

In a preferred embodiment, the present inventors treated the merocyanine compound to each dsRNA extracted from A375 (skin cancer melanoma cells) and CCD-986sk (normal primary skin fibroblast), and measured the rate of change in absorbance at <NUM>. As a result, the average rate of change in absorbance in melanoma cells was higher than that in normal cells, which confirmed that the average rate of change in absorbance in melanoma cells was higher than that in normal cells (see <FIG>).

Therefore, the present disclosure can provide information for the diagnosis of cancer by distinguishing cancer cells from normal cells by measuring the expression level of dsRNA extracted from a sample of a test subject.

The measurement of the expression level of dsRNA in step <NUM>) can be performed by RT-PCR or UV-Vis spectroscopy, but not always limited thereto. Particularly, the expression level of dsRNA can be measured by extracting total RNA from a sample of a test subject, synthesizing cDNA, and then performing RT-PCR with a primer capable of amplifying dsRNA. Or, the measurement can be performed by extracting total RNA from a sample of a test subject, and measuring the absorbance changes that appear in response to the merocyanine compound.

Specifically, the measurement of the expression level of dsRNA in step <NUM>) can include the following steps:.

In addition, the measurement of the expression of dsRNA can further include a step of calculating the rate of change in absorbance by comparing the absorbance of step iv) with that of the reaction solution without dsRNA. The reactivity to the anticancer agent can be predicted according to the calculated rate of change in absorbance. According to an embodiment of the present invention, the expression level of dsRNA in cancer cells that are highly responsive to the anticancer agent can be higher than the expression level of dsRNA in cancer cells that are not responsive to the anticancer agent.

In a preferred embodiment, the inventors treated <NUM>-AZA-CdR (<NUM>-aza-<NUM>'-deoxycytidine, Decitabine), a DNA demethylating agent, to HeLa cervical cancer cells known to not respond to <NUM>-AZA-CdR and HCT116 colorectal cancer cells known to respond to <NUM>-AZA-CdR, separated dsRNA, added the merocyanine compound thereto, and measured the rate of change in absorbance at <NUM>. As a result, the rate of change in absorbance was almost unchanged in HeLa cervical cancer cells, whereas the rate of change in absorbance was increased from day <NUM> of the <NUM>-AZA-CdR treatment in HCT116 cells (see <FIG>).

The present inventors measured the rate of change in absorbance at <NUM> after adding the merocyanine compound and dsRNA extracted from HCT116 colorectal cancer cells, PANC1 pancreatic cancer cells, MCF-<NUM> breast cancer cells, A549 lung cancer cells, and A375 melanoma cells. As a result, it was confirmed that the rate of change in absorbance was increased from day <NUM> of the <NUM>-AZA-CdR treatment in HCT116 cells. It was also confirmed that the expression of dsRNA was slightly increased on day <NUM> of the treatment in PANC-<NUM> pancreatic cancer cells and MCF-<NUM> breast cancer cells compared to day <NUM>. In addition, it was confirmed that there was no change in the expression of dsRNA in A375 melanoma cells almost not killed by <NUM>-AZA-CdR and A549 lung cancer cells (see <FIG>).

The present inventors treated HeLa cervical cancer cells and HCT116 colon cancer cells with <NUM>-AZA-CdR, respectively, and observed apoptosis of each cell. As a result, it was confirmed that apoptosis was not observed in HeLa cervical cancer cells, whereas apoptosis was observed in HCT116 cells (see <FIG>).

The present inventors measured the expression level of ERV in cells treated with <NUM>-AZA-CdR by qPCR, according to the report that <NUM>-AZA-CdR treatment increased ERV (endogenous retroviral element) known to promote apoptosis. As a result, it was confirmed through qPCR that the expression of the ERV THE1B, MTL2B4, MLT1C49 and MER21C genes was increased (see <FIG>).

Therefore, it was confirmed that the reactivity of cancer cells to an anticancer agent can be predicted by measuring the expression level of dsRNA.

Step <NUM>) is as described above. For example, the sample of step <NUM>) can be any one selected from the group consisting of blood, serum, plasma, body fluid, saliva, urine, cells and tissues, but not always limited thereto. In a preferred embodiment of the present invention, the sample can be synovial fluid of a test subject.

In addition, disclosed but not part of the claimed invention is a method for providing information for the diagnosis of Sjogren's syndrome comprising the following steps:.

Step <NUM>) is as described above. For example, the sample of step <NUM>) can be any one selected from the group consisting of blood, serum, plasma, body fluid, saliva, urine, cells and tissues, but not always limited thereto. In a preferred embodiment , the sample can be saliva of a test subject.

In a preferred embodiment, the inventors confirmed that the expression level of dsRNA in a sample isolated from a patient with degenerative joint disease was high (see <FIG>).

The present inventors also confirmed that the expression level of dsRNA in a sample isolated from <NUM> patients with RA-osteoarthritis (OA) disease was high (see <FIG>).

In addition, the present inventors confirmed that the expression level of dsRNA in a sample isolated from a patient with Sjogren's syndrome was higher than that of the normal control group (see <FIG>).

Therefore, it was confirmed that degenerative joint disease or Sjogren's syndrome can be diagnosed by analyzing the expression level of dsRNA.

Hereinafter, the present invention will be described in detail by the following examples.

<NUM> (<NUM> mol) of <NUM>,<NUM>,<NUM>-trimethylindolenine and <NUM> (<NUM> mol) of <NUM>,<NUM>-diiodopropane were dissolved in <NUM> of anhydrous acetonitrile, which was refluxed for <NUM> hours. The mixture was cooled to room temperature, and the precipitate was filtered, washed with MeCN and CHCl<NUM> and dried. As a result, <NUM> of a grayish yellow solid was obtained (yield: <NUM>%).

<NUM>H NMR (<NUM>, DMSO-d<NUM>) δ <NUM>-<NUM> (<NUM>, m), <NUM>-<NUM> (<NUM>, m), <NUM>-<NUM> (<NUM>, m), <NUM>-<NUM> (<NUM>, t), <NUM>-<NUM> (<NUM>, t), <NUM> (<NUM>, s), <NUM>-<NUM> (<NUM>, m), <NUM> (<NUM>, s).

Under nitrogen atmosphere, <NUM> (<NUM> mol) of the <NUM>-(<NUM>-iodopropyl)-<NUM>,<NUM>,<NUM>-trimethylindolinium iodide prepared in step <NUM> was suspended in <NUM> of degassed water, to which <NUM> (<NUM> mol) of finely ground NaOH was added. The reaction solution was heated at <NUM> for <NUM> minutes, and then cooled at room temperature, to which <NUM> of ethyl ether was added. The mixture was stirred for another hour, and the aqueous layer was separated and washed with <NUM> of ethyl ether and <NUM> of dichloromethane. The organic layer was mixed, washed with water, dried over MgSO<NUM> and concentrated in vacuo. As a result, <NUM> of a pink solid was obtained (yield: <NUM>%).

<NUM>H NMR (<NUM>, CDCl<NUM>) δ <NUM>-<NUM> (<NUM>, t), <NUM>-<NUM> (<NUM>, t), <NUM>-<NUM> (<NUM>, d), <NUM>-<NUM> (<NUM>, m), <NUM>-<NUM> (<NUM>, m), <NUM>-<NUM> (<NUM>, m), <NUM>-<NUM> (<NUM>, d), <NUM> (<NUM>, s).

The <NUM>-(<NUM>-iodopropyl)-<NUM>,<NUM>-dimethyl-<NUM>-methyleneindoline prepared in step <NUM> was dissolved in <NUM> of anhydrous ethanol, to which <NUM> (<NUM> mol) of <NUM>-nitrosalicylaldehyde was added. The reaction solution was refluxed under nitrogen for <NUM> hours. The solvent was removed in vacuo, and the residue was purified by silica gel column chromatography using hexane/dichloromethane (<NUM>:<NUM>) as an eluent, followed by recrystallization with ethanol/chloroform. As a result, <NUM> of a yellow solid was obtained (yield: <NUM>%).

<NUM>H NMR (<NUM>, CDCl<NUM>) δ <NUM>-<NUM> (<NUM>, m), <NUM>-<NUM> (<NUM>, t), <NUM>-<NUM> (<NUM>, d), <NUM>-<NUM> (<NUM>, d), <NUM>-<NUM> (<NUM>, t), <NUM>-<NUM> (<NUM>, d), <NUM>-<NUM> (<NUM>, d), <NUM>-<NUM> (<NUM>, d), <NUM>-<NUM> (<NUM>, m), <NUM>-<NUM> (<NUM>, m), <NUM>-<NUM> (<NUM>, m), <NUM> (<NUM>, s), <NUM> (<NUM>, s).

A flask containing <NUM> (<NUM> mol) of the <NUM>'-(<NUM>''-iodopropyl)-<NUM>',<NUM>'-dimethyl-<NUM>-nitrospiro[(<NUM>)-<NUM>-benzopyran-<NUM>,<NUM>'-indoline] prepared in step <NUM> was filled with a rubber septum, to which <NUM>% triethylamine dissolved in ethanol was added using a syringe. The reaction solution was stirred in the dark for <NUM> hours at room temperature. Ethanol and excess triethylamine were removed in vacuo. The residue was purified using a column, and the resulting product was suspended in ethyl ether, filtered and dried. As a result, <NUM> of the spiropyran <NUM>'-(<NUM>"-trimethylammoniopropyl)-<NUM>',<NUM>'-dimethyl-<NUM>-nitrospiro[(<NUM>)-<NUM>-benzopyran-<NUM>,<NUM>'-indoline] iodide was obtained (yield: <NUM>%).

<NUM>H NMR (<NUM>, DMSO-d<NUM>) is <NUM> (<NUM>, s), <NUM>-<NUM> (<NUM>, d), <NUM>-<NUM> (<NUM>, d), <NUM>-<NUM> (<NUM>, m), <NUM>-<NUM> (<NUM>, d), <NUM>-<NUM> (<NUM>, t), <NUM>-<NUM> (<NUM>, d), <NUM>-<NUM> (<NUM>, d), <NUM>-<NUM> (<NUM>, m), <NUM>-<NUM> (<NUM>, m), <NUM> (<NUM>, s), <NUM>-<NUM> (<NUM>, m), <NUM> (<NUM>, s), <NUM> (<NUM>, s).

The spiropyran <NUM>'-(<NUM>"-trimethylammoniopropyl)-<NUM>',<NUM>'-dimethyl-<NUM>-nitrospiro[(<NUM>)-<NUM>-benzopyran-<NUM>,<NUM>'-indoline] iodide prepared in Example <NUM> was converted into merocyanine, an isomer of spiropyran, by <NUM> UV irradiation (<FIG>). The merocyanine can be converted back to spiropyran by visible light irradiation.

The interaction of spiropyran (SP) or merocyanine (MC) with dsRNA was confirmed using a UV-Vis spectrometer.

The spiropyran produced in Example <NUM> was prepared as a spiropyran solution (<NUM>), and dsRNA was prepared by ordering <NUM> bp poly GC and poly AU from Bioneer Co. , respectively. After adding <NUM> of poly GC and poly AU to the spiropyran solution, spectral results were obtained using a UV-Vis spectrometer.

As a result, no change in absorbance spectrum was observed in the SP solution added with poly AU and poly GC dsRNA. Therefore, it was confirmed that SP did not bind to dsRNA (<FIG>).

The spiropyran produced in Example <NUM> was prepared as a spiropyran solution (<NUM>), and dsRNA was prepared by ordering <NUM> bp poly GC and poly AU from Bioneer Co. , respectively. After irradiating <NUM> UV to the spiropyran solution for <NUM> minutes, poly GC and poly AU were added, respectively. Then, spectral results were obtained using a UV-Vis spectrometer.

The SP exposed to UV was converted to merocyanine (MC), an open form isomer of SP (<FIG>). The significant change in absorbance spectrum was observed in the MC solution added with poly AU and poly GC dsRNA, respectively (<FIG> and <FIG>). A hypochromic shift and a red shift were observed at the wavelength of <NUM>, and a small but constant increase in absorbance was observed at the wavelength of <NUM>. This explains that MC is converted to protonated MC (MCH+) by intercalation between nucleotide pairs of dsRNA. In addition, when poly GC was added rather than poly AU, the changes in the spectrum such as a pale shift and a red shift appeared to be more prominent, indicating that MC has a high binding capacity to poly GC-rich RNA.

The effect of the ion concentration of the solution on the interaction of MC and dsRNA was investigated.

After converting <NUM> SP to MC in the same manner as described in Experimental Example <<NUM>-<NUM>> in <NUM> sodium ion (Na+) buffer (pH <NUM>) or nuclease-free water without sodium ions (pH <NUM>), poly AU and poly GC were added at the following concentrations, and absorbance was measured (A: poly AU <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>; B: poly GC <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>; C: poly AU <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>; D: poly GC <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>).

As a result, the changes in the absorbance spectra were greater in water (C and D) without sodium ions than in sodium ion buffer (A and B). The above results indicate that sodium ions can interfere with the electrostatic interaction of positively charged MC with dsRNA (<FIG>).

As the interaction between MC and poly GC dsRNA was strong, the spectral change was prominent. The color change of the MC solution according to the binding of MC and poly GC dsRNA was observed.

After adding <NUM> µℓ of poly GC dsRNA or <NUM> µℓ of water to the MC solution (<NUM> µℓ) prepared in Experimental Example <<NUM>-<NUM>>, color change of the MC solution was observed.

As a result, the color of the MC solution was changed from red to colorless (<FIG>) by adding poly GC dsRNA, but the color was not changed by adding the control (<NUM> µℓ of water). The above results indicate that dsRNA can be detected by visually observing the color change of the MC solution (<FIG>).

To confirm the interaction between MC and single nucleotides, spectrum results were obtained in the same manner as described in Experimental Example <<NUM>-<NUM>>, except that <NUM> types of the RNA single nucleotides rCTP, rGTP, rUTP and rATP were used instead of dsRNA in Experimental Example <<NUM>-<NUM>>. At this time, water was used instead of RNA as the control.

As a result, it was confirmed that there was no change in absorbance spectrum in the MC solution added with each single nucleotide RNA nucleic acid, so that the single nucleotide RNA nucleic acid and MC did not bind (<FIG>).

To confirm that the length of dsRNA affects the interaction of MC-dsRNA, spectrum results were obtained in the same manner as described in Experimental Example <<NUM>-<NUM>>, except that <NUM>, <NUM> and <NUM>-mer poly AU dsRNA were used respectively instead of using <NUM>-mer poly AU and poly GC dsRNA in Experimental Example <<NUM>-<NUM>> and they were treated at the concentration of <NUM> per base pair. At this time, water was used instead of RNA as the control.

As a result, the MC solutions added respectively with <NUM>-mer and <NUM>-mer dsRNAs showed almost the same absorbance spectrum pattern, whereas the MC solution added with <NUM>-mer dsRNA showed weak change in absorbance spectrum. Therefore, it was confirmed that MC was effective in detecting dsRNA of <NUM> bp or more (<FIG>).

To compare and quantify the UV-Vis spectral changes induced by dsRNA, the absorbance change rate observed at <NUM> according to the concentration of dsRNA was calculated.

Particularly, spectrum results were obtained in sodium ion buffer and nuclease-free water without sodium ions in the same manner as described in Experimental Examples <<NUM>-<NUM>> and <NUM>, except that the following concentration of dsRNA was used instead of using <NUM> of dsRNA in Experimental Examples <<NUM>-<NUM>> and <NUM> (A: poly AU <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>; poly GC <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>; B: poly AU <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>; poly GC <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>.

As a result, the rate of change in MC absorbance was increased as the concentration of dsRNA was increased, and the rate of change in absorbance was saturated in the high RNA concentration range (<FIG>). As shown in the previous results, the rate of change in absorbance of poly GC ds RNA was greater than that of poly AU dsRNA, and the rate of change in absorbance in nuclease-free water without sodium ions (Figure 6B) was greater than that in sodium ion buffer (Figure 6A). In addition, since the binding of MC-dsRNA caused a very constant change in the spectrum, it was possible to compare the amount of dsRNA between samples by quantifying the change in absorbance of MC.

The SP and MC in the isomer relationship can be converted reversibly to each other by irradiating UV or visible light. To confirm the effect of dsRNA on the reversibility of SP-MC, SP and <NUM> poly AU and poly GC were added to sodium ion buffer, respectively, and absorbance was measured by alternately irradiating the mixture with UV and <NUM> green light in <NUM> cycles at <NUM> minute intervals. At this time, water was used instead of RNA as the control.

As a result, it was confirmed that the reversibility of SP-MC was maintained independently from the presence or absence of dsRNA (<FIG>).

Whether the MC and dsRNA isolated from cells were bound was investigated. Ribosomal RNA (rRNA), which accounts for about <NUM>% of the RNA present in the cell, has a region that forms a hairpin structure, and thus may bind weakly with MC. Therefore, after treating RNase to remove single strand RNA (ssRNA) and hairpin loops, the interaction of MC and dsRNA isolated from cells was confirmed. At this time, water was used instead of RNA as the control.

Particularly, total RNA was isolated from HeLa cervical cancer cells (TRIsure (Bioline)). The isolated total RNA was treated with RNase T1 and RNase A having different substrate specificities respectively, followed by reacting at <NUM> for <NUM> minutes. After confirming the degraded RNA by electrophoresis with the reaction solution treated with each RNase, spectral results were obtained in the same manner as described in Experimental Example <<NUM>-<NUM>>.

As a result, RNase T1, an RNase that breaks down ssRNA and hairpin loops, decomposed most of rRNA and fragmented thereof, leaving only long dsRNA, and RNase A decomposed all types of RNA (<FIG>). The above results were the same in synthetic dsRNA as well as in RNA isolated from real cells. When RNase A was treated to the total RNA isolated from HeLa cervical cancer cells, the absorbance at <NUM> was almost similar to that of the control group. When dsRNA was isolated from total RNA of cells by treatment of RNase T1, the absorbance at <NUM> was decreased (<FIG>). From the above results, it was confirmed that MC formed intercalation with the dsRNA isolated from real cells as well as synthetic dsRNA (poly AU and poly GC), thereby causing the change in absorbance spectrum.

To compare the expression level of dsRNA between cancer cells and normal cells, total RNA was extracted by treating TRIsure reagents (Bioline) to <NUM> types of cancer cell lines (HeLa cervical cancer cells, HCT116 colorectal cancer cells and A549 lung cancer cells) and <NUM> types of normal cell lines (CCD-986sk cells and RPE-<NUM> cells), respectively. The extracted total RNA (<NUM> µg) was treated with RNase T1 (Worthington Inc. ) in a volume of <NUM>/<NUM>, and incubated at <NUM> for <NUM> minutes to remove ssRNA and rRNA. Then, dsRNA was purified using a phenol extraction method. The final concentration of the purified dsRNA was adjusted to <NUM> using tertiary distilled water, to which the spiropyran solution (<NUM>, dissolved in tertiary distilled water) was added. After irradiating UV to the mixture, the rate of change in absorbance at <NUM> was measured for <NUM> minutes. The rate of change in absorbance was calculated in comparison with the control group using tertiary distilled water instead of dsRNA.

As a result, the average rate of change in absorbance in cancer cells was higher than the average rate of change in absorbance in normal cells, indicating that the expression level of dsRNA in cancer cells was higher than that in normal cells (<FIG>).

The expression levels of dsRNA in A375 skin cancer melanoma cells and normal primary skin fibroblasts were compared in the method described in Experimental Example <<NUM>-<NUM>>.

As a result, the average rate of change in absorbance in melanoma cells was higher than the average rate of change in absorbance in normal cells, indicating that the expression level of dsRNA in melanoma cells was higher than that in normal cells (<FIG>).

Cancer cell responsiveness to drug was evaluated through dsRNA expression analysis using <NUM>-AZA-CdR (<NUM>-aza-<NUM>'-deoxycytidine, Decitabine) as a DNA demethylating agent, and HeLa cervical cancer cells, HCT116 colorectal cancer cells, PANC-<NUM> pancreatic cancer cells, MCF-<NUM> breast cancer cells, A549 lung cancer cells and A375 melanoma cells as cancer cell lines.

HCT116 colorectal cancer cells and HeLa cervical cancer cells were treated with <NUM>-AZA-CdR (<NUM>), respectively, and cultured for <NUM> hours. The medium was replaced with fresh medium and the cells were collected on days <NUM>, <NUM>, <NUM> and <NUM> to isolate dsRNA. The rate of change in absorbance of dsRNA in cancer cells was measured in the same manner as described in Experimental Example <NUM>.

In addition, PANC-<NUM> pancreatic cancer cells, MCF-<NUM> breast cancer cells, A549 lung cancer cells and A375 melanoma cells were treated with <NUM>-AZA-CdR (<NUM>), respectively, and cultured for <NUM> hours. The medium was replaced with fresh medium and the cells were collected on days <NUM>, <NUM>, <NUM>, <NUM> and <NUM> to isolate dsRNA. The rate of change in absorbance of dsRNA in cancer cells was measured in the same manner as described in Example <NUM>.

As a result, the rate of change in absorbance at <NUM> in HCT116 colorectal cancer cells was gradually increased with time, but, the rate of change in absorbance in HeLa cervical cancer cells at day <NUM> was almost similar to that of day <NUM> (<FIG>). In PANC-<NUM> pancreatic cancer cells and MCF-<NUM> breast cancer cells, a slight increase in dsRNA expression was observed on day <NUM> compared to day <NUM>, but there was little change in dsRNA expression in A549 lung cancer cells and A375 melanoma cells (<FIG>).

HCT116 colorectal cancer cells, PANC-<NUM> pancreatic cancer cells, MCF-<NUM> breast cancer cells, A549 lung cancer cells and A375 melanoma cells were treated with <NUM>-AZA-CdR in the same manner as described in Experimental Example <<NUM>-<NUM>>, and the degree of apoptosis was measured by MTT assay.

As a result, the growth of HCT116 colorectal cancer cells was reduced by about <NUM>%, the growth of PANC-<NUM> pancreatic cancer cells and MCF-<NUM> breast cancer cells was decreased by about <NUM>%, and the growth of A549 lung cancer cells was decreased by about <NUM>%, compared to that of the untreated control. The growth of A375 melanoma cells was not reduced (<FIG>).

In addition, HCT116 colorectal cancer cells and HeLa cervical cancer cells were treated with <NUM>-AZA-CdR in the same manner as described in Experimental Example <<NUM>-<NUM>>, and the degree of apoptosis was observed under a microscope on day <NUM>.

As a result, apoptosis was not observed in HeLa cervical cancer cells known to not respond to <NUM>-AZA-CdR, but apoptosis induced by <NUM>-AZA-CdR was observed in HCT116 colorectal cancer cells (<FIG>).

The above results suggest that the degree of apoptosis is consistent with the results of the absorbance change rate of Experimental Example <<NUM>-<NUM>>, and it is possible to predict the cancer cell responsiveness to drug by measuring the dsRNA expression level.

According to a recent study, <NUM>-AZA-CdR has been reported to promote apoptosis by increasing untranslated RNA called ERV (endogenous retroviral element), the dsRNA. Thus, whether the expression of ERV (THE1B, MTL2B4, MLT1C49 and MER21C genes) was increased by <NUM>-AZA-CdR treatment was investigated.

Total RNA was isolated from the HCT116 colorectal cancer cells treated with <NUM>-AZA-CdR in the same manner as described in Experimental Example <<NUM>-<NUM>>, to which DNase I was treated, and then cDNA was synthesized using RevertAid reverse transcriptase (Thermo Fisher Scientific). Using the synthesized cDNA as a template, qPCR was performed with the primers in Table <NUM> below.

As a result, the expression levels of THE1B, MTL2B4, MLT1C49 and MER21C, the ERV, were almost unchanged on days <NUM> and <NUM>, but the expression levels began to increase from day <NUM>. In particular, the expression level of MER21C on day <NUM> was increased by <NUM> times compared to that on day <NUM> (<FIG>). These results are consistent with the trends in the absorbance change rate confirmed in Experimental Example <<NUM>-<NUM>>.

To measure the expression level of dsRNA in patients with degenerative joint disease such as osteoarthritis (OA), rheumatoid arthritis (RA) and gout, <NUM>µℓ of synovial fluid was collected from each patient, to which Trizol LS (Thermo Fisher Scientific) was treated, and then total RNA was extracted according to the manufacturer's instructions. After removing DNA by treating the total RNA with DNase I, cDNA was synthesized using a superscript cDNA synthesis kit (Thermo Fisher Scientific). Using the synthesized cDNA as a template, qPCR was performed with the primers in Table <NUM> below.

Even in synovial fluid, where the expression of dsRNA was expected to be low, the expression level of dsRNA in patients with degenerative joint disease was high, and dsRNAs showing the different expression levels in the synovial fluid at the same site were detected. Through this, it was confirmed that the early diagnosis of degenerative joint disease can be performed and the progression of the disease can be grasped by measuring the expression level of dsRNA (<FIG>).

To measure the expression level of dsRNA in <NUM> patients with RA-osteoarthritis (OA), qPCR was performed with the primers in Table <NUM> below using the cDNA synthesized from <NUM>µℓ of synovial fluid of each patient in the same manner as described in Example <<NUM>-<NUM>> as a template.

As a result, the expression of dsRNA was high in all patients, and dsRNAs showing the different expression levels in the synovial fluid at the same site were detected (<FIG>). These results suggest that degenerative joint disease can be diagnosed early by measuring the expression level of dsRNA.

To compare the expressions of ND1 dsRNA, ND4 dsRNA, ND5 dsRNA, ND6 dsRNA, CYTB dsRNA, CO1 dsRNA, CO2 dsRNA and CO3 dsRNA present in the saliva obtained from <NUM> samples each of normal control (control), simple xerostomia patients (SS-) and Sjogren's syndrome (SS+) patients with xerostomia, <NUM> µℓ of saliva was collected, to which RNeasy Protect Saliva Mini Kit (Qiagen) was treated, and then total RNA was extracted according to the manufacturer's instructions. After removing DNA by treating the total RNA with DNase I, cDNA was synthesized using a superscript cDNA synthesis kit (Invitrogen Inc. Using the synthesized cDNA as a template, qPCR was performed with the primers against various mt dsRNA elements shown in Table <NUM> below.

Claim 1:
A method for diagnosis of a disease selected from the group consisting of Sjogren's syndrome, cancer or a degenerative joint disease and comprising the following steps:
<NUM>)measuring the expression level of dsRNA including the steps of:
i) preparing a merocyanine compound (formula <NUM>), an isomer produced by irradiating UV to the spiropyran compound represented by formula <NUM>;
<CHM>
<CHM>
(In formula <NUM> and formula <NUM>, R is - CH<NUM>CH<NUM>CH<NUM>N+(CH<NUM>)<NUM>)
ii) extracting dsRNA by treating RNase T1 to each total RNA extracted from a test subject;
iii) reacting the merocyanine compound of step i) and the dsRNA of step ii);
iv) measuring the absorbance of the reaction solution of step iii); and
<NUM>) comparing the expression level of dsRNA measured in step <NUM>) with that of the normal control group.