The present invention relates to the construction of a protein-responsive shRNA and RNAi control system using an RNP motif.
RNA interference (hereinafter, referred to as RNAi) is a phenomenon in which translation is transiently inhibited by cleaving mRNA in a sequence-specific manner. An approach called knockdown, which causes this RNAi by introducing an RNA duplex such as short hairpin RNA (hereinafter, referred to as shRNA), has been established in various organism species. RNAi has been diffused widely, including study on its application to medical treatment, in a period as short as 10 years from its discovery as the convenient and potent approach of transiently inhibiting gene expression. However, its mechanisms or introduction techniques still remain to be evolved. Moreover, at this time, the theme of RNAi centers on studies for making knockdown strongly effective or the development of delivery techniques for delivering RNA to a site of interest.
Chung et al. have prepared artificial RNA in which the binding site of theophylline known as a caffeine-like low-molecular-weight compound has been introduced in the loop portion of shRNA, and have revealed that RNAi is inhibited in a theophylline concentration-dependent manner (see Non-Patent Document 1).
An object of the present invention is to provide an RNAi control system using RNP for the purpose of newly designing and preparing a translational control mechanism using RNAs or proteins as inhibitors and incorporating such an artificial translational control system into a living body.
The present invention has been achieved for attaining the object. Specifically, according to one embodiment, the present invention relates to an shRNA comprising: a guide strand having a sequence complementary to a target sequence; a passenger strand which forms a duplex with the guide strand; and a linker strand which links the guide strand and the passenger strand, wherein the linker strand comprises an RNP-derived protein-binding motif sequence. In the present specification, this shRNA is also referred to as a sensor shRNA.
It is preferred that the RNP-derived protein-binding motif sequence should be a Box C/D sequence.
According to an alternative aspect, the present invention relates to an RNAi control system comprising: the sensor shRNA; and an RNP-derived protein which specifically binds to a protein-binding motif sequence in the shRNA.
According to an alternative aspect, the present invention relates to an RNAi control system comprising: a vector for expression of the sensor shRNA; and a vector for expression of an RNP-derived protein which specifically binds to a protein-binding motif sequence in the shRNA.
According to a further alternative aspect, the present invention relates to an RNAi control method comprising the steps of: contacting the sensor shRNA with an RNP-derived protein which specifically binds to a protein-binding motif sequence in the shRNA, in a solution; and introducing the solution containing the shRNA and the protein into a cell.
According to a further alternative aspect, the present invention relates to an intracellular RNAi control method comprising the steps of: introducing a vector for expression of the sensor shRNA into a cell; introducing a vector for expression of an RNP-derived protein which specifically binds to a protein-binding motif sequence in the shRNA, into the cell; and causing their expressions from the vector for expression of the shRNA and the vector for expression of the protein.
According to a further alternative aspect, the present invention provides an RNAi control system responsive to a protein expressed in a cell, the system comprising: the sensor shRNA in which RNP-derived protein-binding motif sequence is a sequence specifically binding to the protein expressed in the cell, or a vector for expression of the shRNA, and also provides an RNAi control method responsive to a protein expressed in a cell, the method comprising the step of: introducing the sensor shRNA in which RNP-derived protein-binding motif sequence is a sequence specifically binding to the protein expressed in the cell, or a vector for expression of the shRNA, into a cell.
According to a further alternative aspect, the present invention provides the RNAi control system which controls the expression of an apoptosis regulatory protein wherein the target sequence of the shRNA is Bc1-xL mRNA, and also provides an artificial protein information conversion system using the shRNA, wherein information of a protein specifically binding to an RNP-derived protein-binding motif sequence is converted to information of a protein encoded by an RNA of the target sequence of the shRNA.
As an advantageous effects of the present invention, use of the sensor shRNA described above enables RNAi control such that RNAi is inhibited in a manner dependent on a protein specifically binding to the shRNA. This means that in the presence of the sensor shRNA, use of a particular protein as an input signal can inhibit the RNAi of particular mRNA and relatively increase the amount of proteins expressed from the particular mRNA. The sensor shRNA according to the present invention used in combination with the particular protein is useful in the construction of biosensors for quantifying the expression of intracellular marker proteins without destroying cells or artificial gene circuits capable of activating the translation of proteins of interest in response to the expression level of marker proteins. For example, the present invention produces significant advantageous effects that lead to the treatment of diseases such as cancer or Alzheimer's disease by activating apoptosis-inducing proteins in response to the expression of cancer marker proteins.
Hereinafter, the present invention will be described in detail with reference to embodiments. However, the present invention is not intended to be limited to the description below.
In recent years, various noncoding RNAs that function in vivo have been discovered, and their roles have received attention. However, these RNAs often form a complex with a protein (RNP) in vivo. Thus, artificial RNP has been expected as a novel nanoblock capable of controlling cell functions. Naturally occurring RNP is found to form many complexes using an RNA-protein interaction motif (RNP motif) composed of a relatively short sequence. For example, HIV Rev proteins interact with high affinity with RNA motifs that recognize Rev. Thus, RNP has been expected to be used as a research material for synthetic biology (field in which biological molecules or the systems of life are constituted through the procedures of artificially creating biological molecules to induce new technologies).
To develop a system for controlling the translation of proteins of interest in response to proteins expressed in cells, the present inventors have come up with the idea that RNA interference is controlled using this RNA-protein interaction motif, thereby controlling the translation of proteins of interest. Based on this idea, the present invention has been completed.
According to a first embodiment, the present invention provides an shRNA comprising: a guide strand having a sequence complementary to a target sequence; a passenger strand which forms a duplex with the guide strand; and a linker strand which links the guide strand and the passenger strand, wherein the linker strand comprises an RNP-derived protein-binding motif sequence.
The shRNA according to the first embodiment is schematically shown in
The guide strand 1 may be an RNA nucleotide sequence of approximately 21 bases to 26 bases and may be located at the 3′ end in the shRNA. The guide strand 1 has a sequence complementary to a particular sequence of mRNA to be controlled (hereinafter, referred to as a target sequence). The mRNA to be controlled can be selected appropriately by those skilled in the art according to the purpose. Examples of the mRNA to be controlled include, but not limited to, mRNAs of apoptosis-inducing genes, mRNAs of apoptosis-suppressing genes, and mRNAs of cancer marker genes. More specific examples of the mRNA to be controlled include GFP mRNA, BimEL mRNA, and Bc1-xL mRNA. Moreover, in these mRNAs, a sequence used as the target sequence can be selected appropriately by those skilled in the art by using design software based on information about the constitution and type of its primary gene sequence in view of inhibited off-target effect and the more efficiently inhibited expression of the target gene. The guide strand must be completely complementary to the target sequence. This is to cause the RNAi effect. At least 2 bases of the 3′-terminal in the guide strand 1 may form overhang that does not form complementary strands with the passenger strand. The guide strand 1 is a portion that becomes siRNA after cleavage by Dicer.
The passenger strand 3 may be an RNA nucleotide sequence of approximately 21 bases to 26 bases and may be located at the 5′ end of the shRNA. When the passenger strand 3 is, for example, of 21 bases, bases 3 to 21 from the 3′ end of the passenger strand 3 have a sequence that forms complementary strands with bases 3 to 21 from the 3′ end of the guide strand 1. When the passenger strand 3 is composed of 21 bases, usually, the guide strand is also composed of 21 bases. The numbers of bases constituting the passenger strand 3 and the guide strand 1 may be 22, 23, 24, 25, or 26. In either case, the numbers of bases of the passenger strand 3 and the guide strand 5 are usually equal. Moreover, as shown in
The linker strand 2 serves as a linker between the guide strand 1 and the passenger strand 3. The linker strand 2 may be bound to the 5′ end of the guide strand 1 and the 3′ end of the passenger strand 3. In other words, the linker strand 2 may be a portion that is cleaved off from the guide strand 1 and the passenger strand 3 after cleavage by Dicer. The linker strand 2 may constitute the major part of the nonhybridized loop portion, as shown in the drawing, in the sensor shRNA according to the present invention. A portion of the nonhybridized loop portion may be derived from a portion of the 3′ end of the passenger strand 3. Alternatively, the linker strand 2 may constitute the whole nonhybridized loop portion, and a few bases at the 3′ end of the linker strand 2 and a few bases at the 5′ end of the linker strand 2 may form a portion of the stem portion of the hairpin structure through hybridization therebetween, though this structure is not shown in the drawings.
The linker strand 2 may comprise a base sequence 20 and an RNP-derived protein-binding motif sequence 21. In this context, the base sequence 20 in the present invention refers to a portion of the sequence constituting the linker strand and a portion that is not derived from the RNP-derived protein-binding motif sequence 21. In another embodiment, the linker strand 2 may be composed only of the RNP-derived protein-binding motif sequence 21. When the linker strand 2 comprises the base sequence 20 and the RNP-derived protein-binding motif sequence 21 or when the linker strand 2 is composed only of the RNP-derived protein-binding motif sequence 21, the linker strand 2 may have, in its sequence, a sequence that does not form complementary strands, and this sequence may constitute the loop portion of the shRNA. The sequence that does not form complementary strands may be of 4 to 20 bases, preferably 4 to 11 bases, and the types of the bases are not limited. Preferable examples of the sequence that does not directly form complementary strands include, but not limited to, 5′-AGCAUAG-3′ and 5′-GAAA-3′.
The 3′-terminal 2 bases of the linker strand 2 may form complementary strands with the 3′-terminal 2 bases of the passenger strand 3. Furthermore, bases 3 to 7 bases may from the 3′ end of the linker strand 2 may form complementary strands with bases 1 to 4 from the 5′ end of the linker strand 2. In this case, the number of bases forming complementary strands is 4. However, this number is not limited to 4 and can be determined between 1 and 8 bases.
When the protein-binding motif sequence 21 is introduced to the base sequence 20, the introduction position of the protein-binding motif sequence 21 is not limited and may be a range which maintains recognition by Dicer described later. Moreover, when the linker strand is free from the base sequence, the protein-binding motif sequence 21 can be bound directly to the guide strand 1 and the passenger strand 3.
In this context, examples of the protein-binding motif sequence 21 include nucleotide sequences derived from RNA-protein complex interaction motifs (RNP motifs), and nucleotide sequences mutated from these nucleotide sequences. In the present invention, the nucleotide sequences derived from RNA-protein complex interaction motifs encompass: nucleotide sequences known as the RNA sequences of RNA-protein interaction motifs in known natural RNA-protein complexes; and nucleotide sequences as the RNA sequences of artificial RNA-protein complex interaction motifs obtained by an in-vitro evolution method. The RNA-protein complexes are a large number of associates of proteins and RNAs that have been confirmed in vivo, and are 3D objects having a complicated structure. The nucleotide sequences derived from natural RNA-protein complex interaction motifs are usually composed of approximately 10 to 80 bases and known to form specific binding in a noncovalent manner, i.e., through a hydrogen bond, with a particular amino acid sequence of a particular protein. Such nucleotide sequences derived from natural RNA-protein complex interaction motifs can be selected from Tables 1 and 2 below and the database: http://gibk26.bse.kyutech.acjp/jouhou/image/dna-protein/rna/ma.html that is available on the website. The protein-binding motif sequence 21 as an RNA-protein interaction motif-derived nucleotide sequence preferably used in the present embodiment is a sequence that can be recognized by Dicer described below in detail to cause RNAi when incorporated in the shRNA. For conformational conditions, it is preferred that such a protein-binding motif sequence 21 should form a characteristic RNA tertiary structure comprising nonnatural base pairs and be highly specific for a protein binding to this site. Moreover, it is preferred that the RNA-protein interaction motif should have Kd of, but not limited to, approximately 0.1 nM to approximately 1 μM.
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The nucleotide sequences derived from artificial RNA-protein complex interaction motifs are the RNA nucleotide sequences of RNA-protein interaction motifs in artificially designed RNA-protein complexes. Such nucleotide sequences are usually composed of approximately 10 to 80 bases and designed to form specific binding in a noncovalent manner, i.e., through a hydrogen bond, with a particular amino acid sequence of a particular protein. Examples of such nucleotide sequences derived from artificial RNA-protein complex interaction motifs include, but not limited to, RNA aptamers specifically binding to the apoptosis-inducing protein Bc1-2 family, and RNA aptamers specifically recognizing cancer cell surface antigens. Moreover, nucleotide sequences listed in Table 3 below are also known, and these can also be used as the RNA-protein complex interaction motif-derived nucleotide sequence 2 of the present invention.
The artificial RNA-protein complexes can be prepared by using a molecular design method and an in-vivo evolution method in combination. The in-vivo evolution method can produce aptamers or ribozymes by selecting functional RNAs from molecular libraries having various sequence diversities, and repeating the reactions of amplification and transcription of their genes (DNAs). Thus, RNA-protein interaction motifs adapted to RNP having a functional structure of interest can be extracted in advance from natural RNP molecules by molecular design or prepared artificially by the in-vitro evolution method. In the present embodiment, for the RNA-protein complex interaction motif-derived nucleotide sequence 2, it is preferred that the RNA-protein complex from which the nucleotide sequence is derived should have a dissociation constant Kd of approximately 0.1 nM to approximately 1 μM. Specific examples of the protein-binding motif sequence 21 include a Box CD sequence: 5′-GGGCGUGAUGCGAAAGCUGACCC-3′ (SEQ ID NO: 2), which is a nucleotide sequence binding to L7Ae (SEQ ID NO: 1) (Moore T et al., Structure Vol. 12, pp. 807-818 (2004)) known to participate in RNA modifications such as RNA methylation or pseudouridylation.
The constitution of the shRNA according to the present embodiment can be obtained by molecular design. The sensor shRNA of the present embodiment can be obtained, for example, by introducing a protein-binding motif sequence to a sequence portion forming the linker strand, based on the sequence of known natural or nonnatural shRNA, or by replacing a protein-binding motif sequence for a sequence portion forming the linker strand, based on the sequence of known natural or nonnatural shRNA. In this procedure, the type and introduction position of the protein-binding motif sequence can be determined in view of the appropriate placement of RNP of interest such that the function of the Dicer protein can be inhibited.
Alternatively, the nucleotide sequence of the guide strand can be determined according to the desired target sequence to design the linker strand and the passenger strand by computer-aided molecular modeling. In this procedure, particular attention may be paid to the correct formation of a duplex structure by the guide strand and the passenger strand.
The shRNA according to the first embodiment may be stably present through the formation of the hairpin structure shown in
Thus, the shRNA according to the first embodiment is characterized in that the shRNA in the form shown in the drawing, i.e., in the form in which the protein-binding motif sequence 21 is unbound to the particular protein, functions in the same way as known natural shRNA.
Next, according to the second embodiment, the present invention provides an RNAi control system comprising: the shRNA according to the first embodiment; and an RNP-derived protein which specifically binds to a protein-binding motif sequence in the shRNA.
The shRNA constituting the RNAi control system according to the present embodiment is schematically shown in
The protein 4 shown in
In the state shown in
Next, the states of the shRNA according to the present embodiment and the protein 4 in a system in which these molecules coexist will be described.
The present embodiment is characterized in that when the protein-binding motif sequence 21 on the shRNA specifically bind the protein 4 to form an RNP by specific binding, Dicer fails to recognize the shRNA in this RNP form. As a result, the Dicer fails to cleave the shRNA. Then, it cannot proceed to the next step of RNAi such that mRNA to be controlled is made insusceptible to cleavage. In other words, the coexistence of the shRNA according to the present embodiment with the protein 4 can inhibit RNAi. Moreover, according to the embodiment the protein 4 as input information is transformed to RNAi inhibition as output.
In this context, the system in which the shRNA and the protein 4 coexist may be a mixture of separately prepared shRNA and protein 4 molecules in a medium. Alternatively, a vector for expression of the shRNA molecule may be designed, and a vector for expression of the molecule of the protein 4 may be designed. These vectors may be introduced into the same cell, and their expressions can also be caused to achieve the system in which the shRNA and the protein 4 coexist. The vector design will be described in detail in Examples described later.
The RNAi control system according to the second embodiment of the present invention can achieve the inhibition of shRNA-mediated RNAi in a protein-specific manner.
Next, according to the third embodiment, the present invention relates to an RNAi control method comprising the steps of: contacting the sensor shRNA according to the first embodiment with an RNP-derived protein which specifically binds to a protein-binding motif sequence in the shRNA, in a solution; and introducing the solution containing the shRNA and the protein into a cell. The combination of the sensor shRNA and the protein used in the present embodiment can be selected based on the first and second embodiments to determine their sequences.
In this context, the sensor shRNA can be obtained by an in-vitro synthesis method called in-vitro transcription. Single-stranded DNA in which a 19-base antisense sequence (TATAGTGAGTCGTATTAGC; SEQ ID NO: 3) of a T7 promoter sequence may be bound to the 3′ end of a sequence serving as a template of shRNA is artificially synthesized (Hokkaido System Science Co., Ltd.), and this may be associated with a 19-base T7 promoter sequence (GCTAATACGACTCACTATA (SEQ ID NO: 4)) artificially synthesized in the same way. This associate may be mixed with ribonucleic acids, salts, and T7 RNA polymerase and reacted at 37° C., as specifically described in detail in Examples to obtain the sensor shRNA.
On the other hand, the protein can be obtained by preparing a vector for expression of the protein and causing its expression using E. coli, followed by purification. For example, a vector for expression of L7Ae (SEQ ID NO: 2), which is a protein specifically binding to a Box-C/D motif represented by SEQ ID NO: 1, can be prepared with reference to Nucleic Acid Research, 2003, Vol. 31, No. 3 869-877. One example of the vector for expression of L7Ae (SEQ ID NO: 2) in E. coli is shown in SEQ ID NO: 5.
In the present embodiment, the contacting step may be performed by mixing the thus-prepared sensor shRNA and protein in the same solution system. The mixing of the shRNA and the protein may be performed under physiological conditions involving pH 6.5 to 8.0 and a temperature of 4 to 42° C., preferably pH 7.3 to 7.5 and a temperature of 4 to 37° C. As a result, the shRNA and the protein may specifically interact with each other to form an RNP complex.
RNAi may be inhibited in the presence of Dicer, ATP, and Mg ions and under appropriate physiological conditions, in addition to the conditions described above. Accordingly, in the contacting step, the sensor shRNA and the protein may be mixed to form an RNP complex, and then, the step of introduction into a cell can be carried out. The concentration of the RNP complex introduced into a cell is, for example, 1 nM to 40 nM shRNA, preferably 1 nM to 20 nM shRNA, and a protein concentration of preferably, but not limited to, that about 1 to 10 times the shRNA concentration. The introduction of the RNP complex into a cell can be performed by, but not limited to, transfection using liposomes and can be performed by those skilled in the art using general methods for introduction of an RNP into cells known in the art.
After the introduction of the RNP complex into a cell, the phenomenon described in the first embodiment with reference to
According to the third embodiment of the present invention, RNAi can be inhibited in vitro.
In an modification of the third embodiment, the protein alone can be administered directly to a cell. This modification involves, after the introduction of the protein into a cell, forming an RNP complex of the sensor shRNA and the protein in the cell, and differs in this point from the third embodiment which involves forming an RNP complex and then introducing it into a cell. In this modification, the sensor shRNA can be introduced into the cell before or after the introduction of the protein into the cell. When the sensor shRNA is introduced into the cell before the protein introduction, a vector for expression of the shRNA may be designed such that the expression of the shRNA in this vector introduced into the cell can be controlled using a small molecule such as tetracycline. In this method, the shRNA can be expressed using tetracycline after the protein introduction. When the sensor shRNA is introduced into the cell after the protein introduction, the shRNA may be introduced directly into the cell or a vector for expression of the shRNA may be introduced into the cell. The protein introduced in the cell forms an RNP complex with the sensor shRNA and enables the expression of a gene of interest to be controlled by RNAi in the cell. Thus, the present embodiment seems to be effective in the development of protein drugs or the treatment of diseases such as cancer.
According to the fourth embodiment, the present invention relates to an intracellular RNAi control method comprising the steps of: introducing a vector for expression of the shRNA according to the first embodiment into a cell; introducing a vector for expression of an RNP-derived protein which specifically binds to a protein-binding motif sequence in the shRNA, into the cell; and causing their expressions from the vector for expression of the shRNA and the vector for expression of the protein.
The vector for expression of the sensor shRNA can be prepared based on the primary structure sequence of the sensor shRNA determined as described in the first embodiment. One example of the vector preparation method is shown in
The protein expression vector can be prepared by incorporating a DNA sequence encoding a protein to be expressed, into vectors for mammalian expression. A vector preparation example is shown in
The present embodiment is characterized by introducing the vector for expression of the shRNA and the vector for expression of the protein into the same cell and causing their expressions. The introducing step can be carried out by transfection. Examples of the transfection include, but not limited to, transfection using liposomes, direct injection, electroporation, and a lentiviral transfection method. The amounts of the shRNA expression vector and the protein expression vector introduced into a cell may differ depending on the purpose and are, for example, the amount of the L7Ae protein expression vector ¼ times to 10 times, preferably 1 time to 4 times that of the shRNA expression vector.
According to the fourth embodiment, RNAi can be inhibited by causing the intracellular expressions of the shRNA and the protein. Examples of a practical application of the embodiment include the treatment of cancer. Moreover, an RNAi control system can also be prepared by combining the vector for expression of the sensor shRNA and the protein expression vector used in the present embodiment.
In a modification, shRNA can be designed such that the protein specifically binding to the protein-binding motif sequence shown in
Moreover, in a further modification of this embodiment, shRNA can be designed such that the protein specifically binding to the protein-binding motif shown in
Furthermore, a cancer control system using L7Ae may be constructed. The same promoter as that expressing such a cancer-related protein is incorporated upstream of the L7Ae protein expression vector. As a result, the RNAi function of apoptosis-controlling sensor shRNA comprising Box C/D incorporated in the linker strand can be regulated freely by regulating the expression of L7 in response to the expression of the cancer-related protein.
An shRNA-GFP sequence for EGFP knockdown (shRNA-GFP (59 mer) GGCAUCAAGGUGAACUUCAAGAUCCAGCAUAGGGAUCUUGAAGUUCACCUUGA UGCCAG;
[In-Vitro Synthesis of shRNA]
[shRNA-Box C/D-GFP]
5.25 μL of L7Aer template (100 μM, 5′-CTGGCATCAAGGTGAACTTCAGCATCACGCCCTTTCGGGTCAGCTGAAGTTCACC TTGATGCCTATAGTGAGTCGTATTAGC-3; SEQ ID NO: 13) as template DNA of shRNA, 5.25 μL of T7 sense primer (100 μM, 5′-GCTAATACGACTCACTATA-3; SEQ ID NO: 4), 30 μL of T7 RNA polymerase, 5 μL of 1 mg/mL pyrophosphatase (ROCHE), 1.75 μL of 20 mg/mL BSA, 28 μL of 1 M Hepes-KOH, 14 μL of 1 M MgCl2, 3.5 μL of 1 M DTT, 14 μL of 0.1 M spermidine, 33.6 μL of 0.1 M ATP (the same holds true for CTP and UTP), 8.96 μL of 0.1 M GTP, 89.6 μL of 0.1 M GMP, and 385 μL of ultrapure water were mixed and reacted overnight at 37° C. After the reaction, 10 μL of TURBO DNase was added thereto and reacted at 37° C. for 30 minutes to degrade the template DNA. After the reaction, phenol extraction and chloroform extraction were performed, and the supernatant was charged into a PD-10 column (GE Healthcare) equilibrated with a PD-10 buffer (0.3 M potassium acetate, 15% (v/v) ethanol, pH 6.0), and washed with 3 mL of PD-10 buffer, followed by elution with 500 μL of PD-10 buffer twice. Then, to the eluate, an equal amount of ethanol was added to perform ethanol precipitation. The supernatant was discarded, and the pellet was dried and then dissolved in 20 μL of 5× dye solution (0.25% BPB, 30% glycerol). The solution was layered on a nondenaturing 15% polyacrylamide (1/30 bisacrylamide) gel and electrophoresed at room temperature for 50 minutes for separation. A band with the size of interest was excised, and 500 μL of elution buffer (0.5 M NaCl, 0.1% SDS, 1 mM EDTA) was added thereto, followed by elution overnight at 37° C. Then, a microfilter (22 μm Millex GP) was attached to a 5-mL syringe (TERUMO CORP.), and the eluate was added to the syringe and filtered through the filter. To this filtrate, a 2.5-fold volume of ethanol was added to perform ethanol precipitation. The supernatant was discarded, and the pellet was dried and then dissolved in 22 μL of ultrapure water. After concentration measurement, this solution was used in subsequent experiments.
[shRNA-Box C/D mut-GFP]
5.25 μL of L7AerN template (100 μM, 5′-CTGGCATCAAGGTGAACTTCAGCATGACGCCCTTTCGGGCAGCTGAAGTTCACCT TGATGCCTATAGTGAGTCGTATTAGC-3; SEQ ID NO: 15) as template DNA of shRNA and 5.25 μL of T7 sense primer (100 μM, SEQ ID NO: 4) were used to perform transcription/synthesis and purification in the same way as in shRNA-Box C/D-GFP. The purification product was dissolved in 22 μL of ultrapure water. After concentration measurement, this solution was used in subsequent experiments.
[shRNA-GFP]
5.25 μL of 481P template (100 μM, 5′-CTGGCATCAAGGTGAACTTCAAGATCCCTATGCTGGATCTTGAAGTTCACCTTGA TGCCTATAGTGAGTCGTATTAGC-3; SEQ ID NO: 16) as template DNA of shRNA and 5.25 μL of T7 sense primer (100 μM, SEQ ID NO: 4) were used to perform transcription/synthesis and purification in the same way as in shRNA-Box C/D-GFP. The purification product was dissolved in 22 μL of ultrapure water. After concentration measurement, this solution was used in subsequent experiments.
Plasmids comprising a gene of the L7Ae protein incorporated in pET-28b+, kindly provided by Dr. Huttenhofer were amplified. From a −80° C. glycerol bacterial stock of E. coli BL21 (DE3) pLysS transformed with the pET-28b+L7Ae plasmid (SEQ ID NO: 5), the bacterial cells were inoculated to 5 mL of medium and shaken-cultured overnight at 37° C. Subsequently, the whole amount of the culture solution was inoculated to 500 mL of LB medium containing 50 μg/mL kanamycin and 100 μg/mL chloramphenicol. The bacterial cells were shake-cultured at 37° C. until O.D.600 became 0.6 to 0.7. Then, 500 μL of 1 M IPTG was added (final concentration: 1 mM) thereto for inducing expression, and the cells were shake-cultured overnight at 30° C. The bacterial cells were collected by centrifugation (4° C., 6000 rpm, 20 minutes). After addition of 5 mL of sonication buffer (50 mM Na phosphate, 0.3 M NaCl, 2.5 mM imidazole, pH 8.0), sonication was performed to disrupt the bacterial cells. In this sonication, the procedure of cooling on ice and then irradiation with ultrasonic waves for 15 seconds was repeated 6 times. Then, impurity proteins were denatured at 80° C. for 15 minutes. The supernatant was collected by centrifugation (4° C., 6000 rpm, 20 minutes), and histidine-tagged proteins were purified by the batch method using an Ni-NTA column (Qiagen). Specifically, first, the supernatant and 1 mL of Ni-NTA were mixed and stirred at 4° C. for 1 hour. Then, the mixture was charged into the column and washed twice with 4 mL of wash buffer (50 mM Na phosphate, 0.3 M NaCl, 20 mM imidazole, pH 8.0). Stepwise elution was performed with 1 mL each of 50 mM, 100 mM, 200 mM, and 300 mM imidazole elution buffers (prepared by adding imidazole to 50 mM Na phosphate, 0.3 M NaCl, pH 8.0) in each of two runs. The proteins of interest were confirmed by 15% SDS-PAGE. Subsequently, Microcon YM-3 (Millipore Corp.) was used to concentrate the proteins, followed by buffer replacement by a dialysis buffer (20 mM Hepes-KOH, 1.5 mM MgCl2, 150 mM KCl, 5% glycerol, pH 7.5). Moreover, the protein concentration was determined by the Bradford method using Protein Assay (Bio-Rad Laboratories, Inc.).
The binding between each shRNA and the protein was confirmed as follows: after dilution with a dialysis buffer to bring the protein concentration to concentrations 25 times the final concentrations of 80 to 640 nM, 2 μL of the protein solution with each concentration, 2 μL of 1 μM shRNA-Box C/D-GFP, 6 μL of ultrapure water, and 40 μL of Opti-MEM I (trademark, Invitrogen Corp.) were mixed and left standing at room temperature for 30 minutes to bind shRNA (40 nM) to L7Ae (80 nM, 160 nM, 320 nM, or 640 nM). shRNA-GFP and shRNA-Box C/D mut-GFP were bound to L7Ae in the same way. To each solution, 13 μL of 5× dye solution (0.25% BPB, 30% glycerol) was added and mixed, and 15 μL of this mixed solution was layered on a nondenaturing 15% polyacrylamide (1/30 bisacrylamide) gel and electrophoresed at 250 V at 4° C. for 50 minutes. After the electrophoresis, the gel was stained with SYBR Green for 15 minutes, and bands were confirmed using FLA-7000 (FUJI FILM).
The inhibition of Dicer cleavage of shRNA-Box C/D-GFP and shRNA-Box C/D mut-GFP by L7Ae was confirmed as follows using GTS, Inc. Recombinant Human Dicer Enzyme Kit according to the protocol: first, 0.4 μL of 4 μM shRNA, 2 μL of 4 μM or 8 μM L7Ae, 1 μL of 10 mM ATP, 0.5 μL of 50 mM MgCl2, 4 μL of Dicer Reaction Buffer (GTS, Inc.), 2 μL of 0.5 unit/μL Recombinant Dicer Enzyme, and 0.1 μL of ultrapure water were mixed and reacted at 37° C. for 15 hours. Then, 2 μL of Dicer Stop Solution was added thereto and mixed. To 8 μL of this mixed solution, 2 μL of 5× dye solution was added, and the mixture was layered on a nondenaturing 15% polyacrylamide (1/30 bisacrylamide) gel and electrophoresed at 4° C. for 50 minutes. After the electrophoresis, the gel was stained with SYBR Green, and bands were confirmed using FLA-7000 (FUJI FILM).
[Construction/Synthesis of shRNA Expression Plasmid]
[Synthesis of pENTR/H1/TO-shRNA-Box C/D-GFP (SEQ ID NO: 17)]
5 μL of pENTR L7Aer Top strand (200 μM, 5′-CACCGGCATCAAGGTGAACTTCAGCTGACCCGAAAGGGCGTGATGCTGAAGTTC ACCTTGATGCC-3; SEQ ID NO: 18) as single-stranded DNA containing an shRNA-encoding sequence for insertion to pENTR/H1/TO vectors (Invitrogen Corp.), 5 μL of pENTR L7Aer Bottom strand (200 μM, 5′-AAAAGGCATCAAGGTGAACTTCAGCATCACGCCCTTTCGGGTCAGCTGAAGTTCA CCTTGATGCC-3; SEQ ID NO: 19) as single-stranded DNA containing a complementary strand thereof, 2 μL of 10× Oligo Annealing Buffer (Invitrogen Corp.), and 2 μL of ultrapure water were mixed, incubated at 95° C. for 4 minutes, and then left standing at room temperature for 5 minutes to form a DNA duplex. This duplex is a duplex shown in
[Synthesis of pENTR/H1/TO-shRNA-Box C/D-mut-GFP (SEQ ID NO: 22)]
pENTR/H1/TO-shRNA-Box C/D-mut-GFP was synthesized and purified in the same way as above using 5 μL of pENTR L7AerN Top strand (200 μM, 5′-CACCGGCATCAAGGTGAACTTCAGCTGCCCGAAAGGGCGTCATGCTGAAGTTCAC CTTGATGCC-3; SEQ ID NO: 23) as single-stranded DNA containing an shRNA-encoding sequence for insertion to pENTR/H1/TO vectors (Invitrogen Corp.) and pENTR L7AerN Bottom strand (200 μM, 5′-AAAAGGCATCAAGGTGAACTTCAGCATGACGCCCTTTCGGGCAGCTGAAGTTCAC CTTGATGCC-3; SEQ ID NO: 24) as single-stranded DNA containing a complementary strand thereof, and dissolved by the addition of 55 μL of ultrapure water. After plasmid vector concentration measurement, this was used in subsequent experiments.
[Synthesis of pENTR/H1/TO-shRNA-GFP (SEQ ID NO: 25)]
pENTR/H1/TO-shRNA-GFP was synthesized and purified in the same way as above using 5 μL of pENTR 481P Top strand (200 μM, 5′-CACCGGCATCAAGGTGAACTTCAAGATCCAGCATAGGGATCTTGAAGTTCACCTT GATGCC-3; SEQ ID NO: 26) as single-stranded DNA containing an shRNA-encoding sequence for insertion to pENTR/H1/TO vectors (Invitrogen Corp.) and pENTR 481P Bottom strand (200 μM, 5′-AAAAGGCATCAAGGTGAACTTCAAGATCCCTATGCTGGATCTTGAAGTTCACCTT GATGCC-3; SEQ ID NO: 27) as single-stranded DNA containing a complementary strand thereof, and dissolved by the addition of 55 μL of ultrapure water. After plasmid vector concentration measurement, this was used in subsequent experiments.
[Synthesis of pENTR/H1/TO-shRNA-GFP-mut (SEQ ID NO: 28)]
pENTR/H1/TO-shRNA-GFP-mut was synthesized and purified in the same way as above using 5 μL of pENTR Sk-7N Top strand (200 μM, 5′-CACCGCACTAGCGTATGAATGAAAGATCCAGCATAGGGATCTTTCATTCATACGC TAGTGC-3; SEQ ID NO: 29) as single-stranded DNA containing an shRNA-encoding sequence for insertion to pENTR/H1/TO vectors (Invitrogen Corp.) and pENTR Sk-7N Bottom strand (200 μM, 5′-AAAAGCACTAGCGTATGAATGAAAGATCCCTATGCTGGATCTTTCATTCATACGC TAGTGC-3; SEQ ID NO: 30) as single-stranded DNA containing a complementary strand thereof, and dissolved by the addition of 55 μL of ultrapure water. After plasmid vector concentration measurement, this was used in subsequent experiments.
[Synthesis of pcDNA3.1-L7Ae-myc-His6 (SEQ ID NO: 6)]
PCR was performed using pET-28b+L7Ae (SEQ ID NO: 5) as template DNA and BamHI-NdeI-NotI-L7Ae-primer (5′-AAGGATCCATCATATGCGGCCGCTTATGTACGTGAGATTTGAGG-3′) (SEQ ID NO: 32) and L7Ae-EcoRI-XhoI-primer (5′-CACTCGAGTTGAATTCTCTTCTGAAGGCCTTTAATC-3′) (SEQ ID NO: 33) as primers. 50 μL of this reaction solution contained a mixture of 2.5 μL of 10 ng/μL template DNA, 1.5 μL of each 10 μM DNA primer, 5 μL of 2 mM dNTPs, 5 μL of 10×KOD-PLUS-buffer ver. 2, 2 μL of 25 mM MgSO4, 1 μL of KOD-PLUS-DNA Polymerase, and 31.5 μL of ultrapure water. The reaction was performed by initial incubation at 94° C. for 2 minutes, followed by 36 cycles each involving 98° C. for 10 seconds, 55° C. for 30 seconds, and 68° C. for 1 minute. From the resulting PCR product, DNA was purified using PCR Purification Kit (QIAGEN). However, elution was performed with 30 μL of ultrapure water, and this DNA was used as a template in restriction enzyme treatment. 27 μL of the template, 5 μL of B Buffer (ROCHE), 1 μL of 10 U/μL BamH1 (ROCHE), 1 μL of 10 U/μL XhoI (ROCHE), and 16 μL of ultrapure water were mixed and reacted at 37° C. for 2 hours for restriction enzyme treatment. Also for pcDNA3.1 (+) myc H is A vectors (Invitrogen Corp.), 1.88 μL of 1.6 μg/μL pcDNA vectors, 5 μL of B Buffer, 1 μL of 10 U/μL BamH1, 1 μL of 10 U/μL XhoI, and 41.12 μL of ultrapure water were mixed, and restriction enzyme treatment was performed in the same way. These treatment products were purified using PCR Purification Kit (QIAGEN). However, for elution, DNA was eluted into 10 μL of ultrapure water.
1.75 μL of the PCR product thus subjected to restriction enzyme treatment, 0.25 μL of the vectors thus subjected to restriction enzyme treatment, and 2 μL of Ligation High were mixed and incubated at 16° C. for 30 minutes. To the whole amount of this ligation reaction solution, 20 μL of Top10 Chemically competent cells (Invitrogen Corp.) was added. The cells were left standing on ice for 45 minutes, then placed in water bath at 42° C. for 1 minute, and left standing again on ice for 2 minutes for transformation. After further addition of 160 μL of LB medium, the cells were seeded over an LB plate containing 50 μg/mL ampicillin and incubated overnight at 37° C. The formed colonies were subjected to colony PCR using Extaq (TAKARA BIO INC.) and the DNA primers described above to check the insert. A colony in which the insert was confirmed was inoculated to 50 mL of LB medium containing 50 μg/mL ampicillin and shake-cultured overnight at 37° C. The bacterial cells were collected by centrifugation (4° C., 6000 rpm, 15 minutes) and purified according to the protocol of Plasmid Purification Kit (Qiagen), followed by isopropanol precipitation. The supernatant was discarded, and the pellet was dried and then dissolved by the addition of 55 μL of ultrapure water. After plasmid vector concentration measurement, this plasmid vector was sequenced using T7 promoter primer (5′-TAATACGACTCACTATAGGG-3; SEQ ID NO: 34) and BGH rev primer (5′-GCTGGCAACTAGAAGGCACAG-3; SEQ ID NO: 35) and used in subsequent experiments.
On the day before transfection, HeLa cells were seeded over a 24-well plate at a concentration of 0.8×105 cells/well and cultured in a CO2 incubator at 37° C. On the next day, the cells were cotransfected with each pENTR/H1/TO shRNA expression vector, pcDNA3.1-AsRed2-L7Ae-myc-His6 (SEQ ID NO: 40), and pcDNA3.1-EGFP-myc-His6 (SEQ ID NO: 41) using Lipofectamine 2000 (Invitrogen Corp.) (trademark). To 0.3 μg each of pENTR-shRNA-GFP, pENTR-shRNA-GFP mut, pENTR-shRNA-Box C/D-GFP, and pENTR-shRNA-Box C/D mut-GFP, 0.3 μg of pcDNA3.1-AsRed2-L7Ae-myc-His6 or pcDNA3.1-AsRed2-myc-His6 (SEQ ID NO: 42) and 0.2 μg of pcDNA3.1-EGFP-myc-His6 were added, and 1.25 μl of Lipofectamine 2000 was added per sample. These DNA-lipid complexes were incubated at room temperature for 20 minutes and added dropwise to the medium for HeLa cells. 4 hours later, medium replacement was performed. 24 hours later, the fluorescence microscope image of the cells was obtained using a fluorescence microscope (OLYMPUS IX-81) to observe the inhibition of shRNA-Box C/D-GFP function by AsRed2-L7Ae expression.
Change in GFP mRNA level caused by RNAi control by L7Ae was determined by real-time PCR.
On the previous day, HeLa-GFP cells were seeded over a 6-well plate at a concentration of 0.5×106 cells/well and cultured in a CO2 incubator at 37° C. Then, the cells were cotransfected with each pENTR/H1/TO shRNA expression vector and pcDNA3.1-L7Ae-myc-His6. To 4 μg each of pENTR-shRNA-Box C/D-GFP and pENTR-shRNA-Box C/D mut-GFP, 0, 2, or 4 μg of pcDNA3.1-L7Ae-myc-His6 was added, and 5 μl of Lipofectamine 2000 was added per sample. These DNA-lipid complexes were incubated at room temperature for 20 minutes and added dropwise to the cells. 4 hours later, medium replacement was performed. 24 hours after the transfection, the cells were collected, and RNA extraction and DNA removal were performed using RNAqueous 4PCR Kit (Ambion, Inc. (trademark)).
1.5 μg (or 0.5 μg) of the extracted RNA was used as a template to synthesize cDNA using High-Capacity cDNA Reverse Transcription Kits (Applied Biosystems Inc. (trademark)), random primers, and reverse transcriptase. Real-time PCR was performed using 1/20-diluted cDNA as a template and LightCycler 480 Taqman probe (Roche) (trademark). PCR reaction and real-time fluorescence detection were carried out using LightCycler 480 (Roche) (trademark). The reaction conditions involved an initial denaturation step at 95° C. for 5 minutes and an amplification step of 45 cycles each involving denaturation at 95° C. for 10 seconds and annealing/elongation at 60° C. for 25 seconds. Finally, the reaction solution was cooled at 50° C. for 15 seconds to terminate the measurement. The Ct value was determined by the Abs Quant/fit point method. The GFP gene of interest was amplified using 481P Fwd (5′-CAAGGAGGACGGCAACA-3′) (SEQ ID NO: 36) and Rev (5′-CCTTGATGCCGTTCTTCTGC-3′) (SEQ ID NO: 37). A reference gene GAPDH was amplified using GAPDH Fwd (5′-AGCCACATCGCTCAGACAC-3′) (SEQ ID NO: 38) and GAPDH Rev (5′-GCCCAATACGACCAAATCC-3′) (SEQ ID NO: 39). The amplification efficiency of GFP mRNA and GAPDH mRNA was determined using Universal probe Library probe #148 (ROCHE) and Universal probe Library probe #60 (ROCHE), respectively. The amplification product was confirmed by electrophoresis to be the single product of interest, and the results were evaluated by relative quantification. The EGFP level was normalized with GAPDH, and this normalized value was used in comparison among samples with the GFP mRNA relative level of a sample supplemented only with pENTR-shRNA-GFP mut as 1.
On the day before transfection, HeLa-GFP cells were seeded over a 24-well plate at a concentration of 0.5×105 cells/well and cultured in a CO2 incubator at 37° C. On the next day, the cells were cotransfected with each pENTR/H1/TO shRNA expression vector and pcDNA3.1-L7Ae-myc-His6 using Lipofectamine 2000 (Invitrogen Corp.) (trademark). To 0.8 μg each of pENTR-shRNA-Box C/D-GFP and pENTR-shRNA-Box C/D mut-GFP, 0, 0.40, or 0.80 μg of pcDNA3.1-L7Ae-myc-His6 was added, and 2 μl of Lipofectamine 2000 was added per sample. These DNA-lipid complexes were incubated at room temperature for 20 minutes and added dropwise to the cells. 4 hours later, medium replacement was performed.
24 hours after the transfection, the medium in each well was removed, and the cells were dissociated using 200 μl of Trypsin-EDTA and suspended by the addition of 200 μl of DMEM/F12. The cell suspension was transferred to a FACS tube and analyzed using FACSAria (BD). In this context, live cells were gated, and FITC was determined for 20000 cells. The analysis was conducted using a general method comprising calculating a mean value of the fluorescence intensities of all the measured cells.
shRNA-U1A-4 for EGFP knockdown (5′-GGCAUCAAGGUGAACUUCAGGGCGAAAGCCCUGAAGUUCACCUUGAUGCCAG-3; SEQ ID NO: 14) was designed. The shRNA-U1A-4 comprised: 5′-terminal 24 bases which were the same as those in the passenger strand of shRNA-GFP shown in
[In-Vitro Synthesis of shRNA]
[shRNA-U1A-4]
5.25 μL of template single-stranded DNA of shRNA-U1A-4 (100 μM, 5′-CTGGCATCAAGGTGAACTTCAGGGCTTTCGCCCTGAAGTTCACCTTGATGCCTAT AGTGAGTCGTATTAGC-3′ SEQ ID NO: 31) and 5.25 μL of T7 sense primer (SEQ ID NO: 4) were used to perform transcription/synthesis and purification in the same way as in shRNA-Box C/D-GFP. The purification product was dissolved in 22 μL of ultrapure water. After concentration measurement, this solution was used in subsequent experiments.
[shRNA-Box C/D-GFP]
It was produced according to the in-vitro synthesis method described in Example 1.
It was produced according to the L7Ae protein expression and purification using E. coli described in Example 1.
On the day before transfection, HeLa-GFP cells were seeded over a 24-well plate at a concentration of 0.5×105 cells/well and cultured in a CO2 incubator at 37° C. In this context, the HeLa-GFP cell strain was HeLa cells in which GFP was stably expressed in a hygromycin-resistant manner, and was kindly provided by Dr. T. Suzuki. On the next day, the medium in the 24 wells was replaced by 500 μl of Opti-MEM (Invitrogen Corp.). At the same time, complexes of shRNA-Box C/D-GFP and the L7Ae protein were introduced into the cells by transfection using Lipofectamine 2000 (Invitrogen Corp.) (trademark). 0.6 μl of 10 μM shRNA-Box C/D-GFP, 0 μl, 0.6 μl, 1.2 μl, 2.4 μl, 4.8 μl, or 9.6 μl of 20 μM L7Ae protein, and 2 μl of 5× binding buffer were mixed, and ultrapure water was added thereto to bring the whole amount to 10 μl (for 9.6 μl of the L7Ae protein, the whole amount was brought to 12.2 μl without the addition of ultrapure water). 40 μl (for 9.6 μl of the L7Ae protein, 37.8 μl) of Opti-MEM was further added thereto and mixed, and the mixture was left standing at 4° C. for 30 minutes to form RNA-protein complexes. 48 μl of Opti-MEM and 2 μl of Lipofectamine 2000 were mixed and left standing at room temperature for 5 minutes. To this mixture, 50 μl of the RNA-protein complex solution was added and mixed, and the mixture was left standing at room temperature for 20 minutes to form RNA-protein-lipid complexes, which were in turn added dropwise to the cells. 4 hours later, the medium was replaced by 500 μl of DMEM/F12. An shRNA-free molecule (Mock) and shRNA-U1A-4 were mixed with the L7Ae protein in the same way to form RNA-protein complexes, which were in turn introduced into the cells by transfection.
45 hours after the transfection, the cells were observed under a fluorescence microscope. The intracellular GFP fluorescence was photographed with settings of 20× magnification and 488 nM excitation wavelength on a fluorescence microscope (OLYMPUS) per sample. At the same time, a phase-contrast image of the cells was also taken using transmitted light.
47 hours after the transfection, the medium in each well was removed, and the cells were dissociated using 200 μl of Trypsin-EDTA and suspended by the addition of 200 μl of DMEM/F12. The cell suspension was transferred to a FACS tube and analyzed using FACSAria (BD). The FACS is a method comprising irradiating, with laser light, free cells passing through a thin tube and analyzing the intensity of fluorescence emitted from the cells. In this context, live cells were gated, and FITC was determined for 10000 cells.
shRNA-Box C/D-Bc1-xL (
[Synthesis of shRNA]
[shRNA-Box C/D-Bc1-xL (
5.25 μL of shRNA-Box C/D-Bc1xL template (100 μM, 5′-CTGCTTTGAACAGGTAGTGAATGATCACGCCCTTTCGGGTCACATTCACTACCTGT TCAAAGCTATAGTGAGTCGTATTAGC-3′ (SEQ ID NO: 44)) as template DNA of shRNA and 5.25 μL of T7 sense primer (100 μM, 5′-GCTAATACGACTCACTATA-3′ (SEQ ID NO: 4)) were used to perform transcription/synthesis and purification in the same way as in shRNA-Box C/D-GFP. The purification product was dissolved in 22 μL of ultrapure water. After concentration measurement, this solution was used in subsequent experiments.
[shRNA-Box C/D mut-Bc1-xL (
5.25 μL of shRNA-Box C/D mut-Bc1xL template (100 μM, 5′-CTGCTTTGAACAGGTAGTGAATGATGACGCCCTTTCGGGCACATTCACTACCTGTT CAAAGCTATAGTGAGTCGTATTAGC-3′ (SEQ ID NO: 46)) as template DNA of shRNA and 5.25 μL of T7 sense primer (100 μM, 5′-GCTAATACGACTCACTATA-3′ (SEQ ID NO: 4)) were used to perform transcription/synthesis and purification in the same way as in shRNA-Box C/D-GFP. The purification product was dissolved in 22 μL of ultrapure water. After concentration measurement, this solution was used in subsequent experiments.
[shRNA-Bc1-xL (
5.25 μL of shRNA-Bc1-xL template (100 μM, 5′-CTGCTTTGAACAGGTAGTGAATGAACTCTATGCTAGTTCATTCACTACCTGTTCAA AGCTATAGTGAGTCGTATTAGC-3′ (SEQ ID NO: 48)) as template DNA of shRNA and 5.25 μL of T7 sense primer (100 μM, 5′-GCTAATACGACTCACTATA-3′ (SEQ ID NO: 4)) were used to perform transcription/synthesis and purification in the same way as in shRNA-Box C/D-GFP. The purification product was dissolved in 22 μL of ultrapure water. After concentration measurement, this solution was used in subsequent experiments.
[Confirmation of knockdown of Bc1-xL by shRNA-Bc1-xL]
On the day before transfection, HeLa-GFP cells were seeded over a 24-well plate at a concentration of 0.5×105 cells/well and cultured in a CO2 incubator at 37° C. On the next day, the cells were cotransfected with Bc1-xL, expression vectors, and shRNA using Lipofectamine 2000 (Invitrogen Corp.). 0 or 0.4 μg of pBc1-xL and 10 μM shRNA-Bc1-xL were mixed and brought to 50 μl with Opti-MEM I medium (Invitrogen Corp.). Then, a mixture of 1 μl of Lipofectamine 2000 supplemented with 49 μl of Opti-MEM I medium was added per sample. These DNA-lipid complexes were incubated at room temperature for 20 minutes. After addition of 400 μl of Opti-MEM I medium, the mixture was added dropwise to the cells. 4 hours later, medium replacement was performed.
24 hours after the transfection, the medium in each well was collected. Then, the cells were dissociated using 200 μl of Trypsin-EDTA and suspended by the addition of each medium collected in the previous step. The cell suspension was subjected to centrifugal sedimentation at 500×g at 4° C. for 5 minutes and washed with 500 μl of PBS. Then, to the cell pellet, 30 μl of RIPA buffer (1×PBS, 1% NP40, 0.5% Sodium deoxycholate, 0.1% SDS, 0.3 mg/ml PMSF+2 μg/ml Aprotinin) was added, and the mixture was left standing on ice for 30 minutes. The supernatant was collected by centrifugation (4° C., 15000 g, 20 minutes). The protein concentration was determined by the Lowry method using DC-Protein Assay (Bio-Rad Laboratories, Inc.).
Bc1-xL was detected by western blotting. Proteins extracted from the cells were developed by SDS-PAGE and subjected to western blotting. A primary antibody Anti-Bc1-xL (SC-634) (Santa Cruz Biotechnology, Inc.) (1/500) and a secondary antibody Goat Anti-Rabbit IgG (H+L)-HRP conjugate (Bio-Rad Laboratories, Inc.) (1/2000) were used. Color was developed using ECL Plus (GE Healthcare) (trademark) and detected using LAS3000 (FUJI FILM). By virtue of the cotransfection of shRNA-Bc1-xL with pBc1-xL, a band showing the expression of Bc1-xL did not appear. The results demonstrated Bc1-xL knockdown by shRNA-Bc1-xL in the HeLa cells.
The inhibition of Dicer cleavage of shRNA-Box C/D-Bc1-xL and shRNA-Box C/D mut-Bc1-xL by L7Ae was confirmed as follows using GTS, Inc. Recombinant Human Dicer Enzyme Kit according to the protocol: first, 0.4 μL of 1 μM shRNA, 2 μL of 4 μM or 8 μM L7Ae, 1 μL of 10 mM ATP, 0.5 μL of 50 mM MgCl2, 4 μL of Dicer Reaction Buffer (GTS, Inc.), 2 μL of 0.5 unit/μL Recombinant Dicer Enzyme, and 0.1 μL of ultrapure water were mixed and reacted at 37° C. for 14 hours. Then, 2 μL of Dicer Stop Solution was added thereto and mixed. To 8 μL of this mixed solution, 2 μL of 5× dye solution was added, and the mixture was layered on a nondenaturing 15% polyacrylamide (1/30 bisacrylamide) gel and electrophoresed at 4° C. for 50 minutes. After the electrophoresis, the gel was stained with SYBR Green, and bands were confirmed using FLA-7000 (FUJI FILM).
Construction/Synthesis of shRNA Expression Plasmid
[Synthesis of pENTR/H1/TO-shRNA-Box C/D-Bc1-xL (SEQ ID NO: 49)]
pENTR/H1/TO-shRNA-Box C/D-Bc1-xL was synthesized and purified in the same way as above using 5 μL of Box C/D Bc1-xL Top strand (200 μM, 5′-CACCGCTTTGAACAGGTAGTGAATGTGACCCGAAAGGGCGTGATCATTCACTACC TGTTCAAAGC-3′ (SEQ ID NO: 50)) as single-stranded DNA containing an shRNA-encoding sequence for insertion to pENTR/H1/TO vectors (Invitrogen Corp.) and Box C/D Bc1-xL Bottom strand (200 μM, 5′-AAAAGCTTTGAACAGGTAGTGAATGATCACGCCCTTTCGGGTCACATTCACTACC TGTTCAAAGC-3′ (SEQ ID NO: 51)) as single-stranded DNA containing a complementary strand thereof, and dissolved by the addition of 55 μL of ultrapure water. After plasmid vector concentration measurement, this was used in subsequent experiments.
[Synthesis of pENTR H1 TO-shRNA-Box C/D mut-Bc1-xL (SEQ ID NO: 52)]
pENTR/H1/TO-Box C/D mut-Bc1-xL was synthesized and purified in the same way as above using 5 μL of Box C/D mut Bc1-xL Top strand (200 μM, 5′-CACCGCTTTGAACAGGTAGTGAATGTGCCCGAAAGGGCGTCATCATTCACTACCT GTTCAAAGC-3′ (SEQ ID NO: 53)) as single-stranded DNA containing an shRNA-encoding sequence for insertion to pENTR/H1/TO vectors (Invitrogen Corp.) and Box C/D mut Bc1-xL Bottom strand (200 μM, 5′-AAAAGCTTTGAACAGGTAGTGAATGATGACGCCCTTTCGGGCACATTCACTACCT GTTCAAAGC-3′ (SEQ ID NO: 54)) as single-stranded DNA containing a complementary strand thereof, and dissolved by the addition of 55 μL of ultrapure water. After plasmid vector concentration measurement, this was used in subsequent experiments.
[Synthesis of pENTR/H1/TO-shRNA-Bc1-xL (SEQ ID NO: 55)]
pENTR/H1/TO-shRNA-Bc1-xL was synthesized and purified in the same way as above using 5 μL of Bc1-xL Top strand (200 μM, 5′-CACCGCTTTGAACAGGTAGTGAATGAACTAGCATAGAGTTCATTCACTACCTGTT CAAAGC-3′ (SEQ ID NO: 56)) as single-stranded DNA containing an shRNA-encoding sequence for insertion to pENTR/H1/TO vectors (Invitrogen Corp.) and Bc1-xL Bottom strand (200 μM, 5′-AAAAGCTTTGAACAGGTAGTGAATGAACTCTATGCTAGTTCATTCACTACCTGTT CAAAGC-3′ (SEQ ID NO: 57)) as single-stranded DNA containing a complementary strand thereof, and dissolved by the addition of 55 μL of ultrapure water. After plasmid vector concentration measurement, this was used in subsequent experiments.
To confirm the control of Bc1-xL knockdown by the binding between the L7Ae protein and shRNA-Box C/D-Bc1-xL in cultured human cancer cells, RNA-protein complexes were introduced into the cells, and the expression of Bc1-xL was detected by western blotting.
On the previous day, uterine cervix cancer-derived HeLa cells were seeded over a 24-well plate at a concentration of 1.0×105 cells/well and cultured in a CO2 incubator at 37° C. On the next day, transfection was performed twice using Lipofectamine 2000 (Invitrogen Corp.) (trademark). To 0.4 μg of pBc1-xL or pBimEL, 1 μl of Lipofectamine 2000 was added. These DNA-lipid complexes were incubated at room temperature for 20 minutes and added dropwise to the medium for HeLa cells. 4.5 hours later, medium replacement was performed. Immediately thereafter, the second transfection was performed. 2.5 pmol (concentration in the medium: 5 nM) of shRNA-Box C/D-Bc1-xL or shRNA-Box C/D mut-Bc1-xL and 0 or 200 pmol (concentration in the medium: 400 nM) of the purified L7Ae protein were mixed to form complexes. To the complexes, 1 μl of Lipofectamine 2000 was added, and the complexes were incubated at room temperature for 20 minutes and added dropwise to the medium for HeLa cells. 5 hours later, medium replacement was performed.
22 hours after the second transfection, the medium in each well was collected. Then, the cells were dissociated using 200 μl of Trypsin-EDTA and suspended by the addition of each medium collected in the previous step. The cell suspension was subjected to centrifugal sedimentation at 500× g at 4° C. for 5 minutes and washed with 500 μl of PBS. Then, to the cell pellet, 30 μl of RIPA buffer (1×PBS, 1% NP40, 0.5% Sodium deoxycholate, 0.1% SDS, 0.3 mg/ml PMSF+2 g/ml Aprotinin) was added, and the mixture was left standing on ice for 30 minutes. The supernatant was collected by centrifugation (4° C., 15000× g, 20 minutes). The protein concentration was determined by the Lowry method using DC-Protein Assay (Bio-Rad Laboratories, Inc.).
Bc1-xL or GAPDH was detected by western blotting. Proteins extracted from the cells were developed by SDS-PAGE and subjected to western blotting. A primary antibody Anti-Bc1-xL (SC-634) (Santa Cruz Biotechnology, Inc.) (1/500) and a secondary antibody Goat Anti-Rabbit IgG (H+L)-HRP conjugate (Bio-Rad Laboratories, Inc.) (1/2000) were used. Color was developed using ECL Plus (GE Healthcare) (trademark) and detected using LAS3000 (FUJI FILM). Likewise, GAPDH was subjected to western blotting using a primary antibody Anti-GAPDH (MAB374) (Chemicon International, Inc.) (1/2000) and a secondary antibody Goat Anti-Mouse IgG (H+L)-HRP conjugate (Bio-Rad Laboratories, Inc.) (1/2000). These results demonstrated that Bc1-xL knockdown was inhibited (lane 3) by the binding between the L7Ae protein and shRNA-Box C/D-Bc1-xL in the HeLa cells. Protein extraction from cells and L7Ae detection shown below were performed in the same way.
To confirm the control of Bc1-xL knockdown by the binding between the L7Ae protein and shRNA-Box C/D-Bc1-xL in cultured human cancer cells, the cells were cotransfected with plasmids for expressions of Bc1-xL, L7Ae, and shRNA, and the expression of Bc1-xL was detected by western blotting.
On the previous day, uterine cervix cancer-derived HeLa cells were seeded over a 12-well plate at a concentration of 3.0×105 cells/well and cultured in a CO2 incubator at 37° C. On the next day, transfection was performed using Lipofectamine 2000 (Invitrogen Corp.) (trademark). 0.2 μg of pBc1-xL, 0.4 μg of pcDNA3.1-L7Ae, and 0.6 μg of pENTR/H1/TO-shRNA-Box C/D-Bc1-xL were mixed, and 2.5 μl of Lipofectamine 2000 was added thereto. These DNA-lipid complexes were incubated at room temperature for 20 minutes and added dropwise to the medium for HeLa cells. For pENTR/H1/TO-shRNA-Box C/D-mut Bc1-xL, pENTR/H1/TO-shRNA-Bc1-xL, and pENTR/H1/TO-shRNA-GFP mut (negative control), the same procedures were also performed. 0.25 μg of pcDNA-AmCyan-myc-His6 ((SEQ ID NO: 58) or 0.2 μg of pBc1-xL were introduced alone as a control plasmid into the cells. 4 hours later, medium replacement was performed.
24 hours after the transfection, the medium in each well was collected. Then, the cells were dissociated using 200 μl of Trypsin-EDTA and suspended by the addition of each medium collected in the previous step. The cell suspension was subjected to centrifugal sedimentation at 500× g at 4° C. for 5 minutes and washed with 500 μl of PBS. Then, to the cell pellet, 100 μl of RIPA buffer (1×PBS, 1% NP40, 0.5% Sodium deoxycholate, 0.1% SDS, 0.3 mg/ml PMSF+2 μg/ml Aprotinin) was added, and the mixture was left standing on ice for 30 minutes. The supernatant was collected by centrifugation (4° C., 15000 g, 20 minutes). The protein concentration was determined by the Lowry method using DC-Protein Assay (Bio-Rad Laboratories, Inc.).
Bc1-xL or GAPDH was detected by western blotting. Proteins extracted from the cells were developed by SDS-PAGE and subjected to western blotting. A primary antibody Anti-Bc1-xL (SC-634) (Santa Cruz Biotechnology, Inc.) (1/500) and a secondary antibody Goat Anti-Rabbit IgG (H+L)-HRP conjugate (Bio-Rad Laboratories, Inc.) (1/2000) were used. Color was developed using ECL Plus (GE Healthcare) (trademark) and detected using LAS3000 (FUJI FILM). Likewise, GAPDH was subjected to western blotting using a primary antibody Anti-GAPDH (MAB374) (Chemicon International, Inc.) (1/2000) and a secondary antibody Goat Anti-Mouse IgG (H+L)-HRP conjugate (Bio-Rad Laboratories, Inc.) (1/2000). These results demonstrated that Bc1-xL knockdown was inhibited (lane 5) by the binding between the L7Ae protein and shRNA-Box C/D-Bc1-xL in the HeLa cells.
An apoptosis-promoting protein Bim-EL and an apoptosis-suppressing protein Bc1-xL have antagonistic effect on each other, and a relatively larger amount of the protein affects the fate of cells. Thus, an experiment was conducted which involved controlling Bc1-xL expression levels using the control of Bc1-xL knockdown by the binding between the L7Ae protein and shRNA-Box C/D-Bc1-xL in cultured human cancer cells, and controlling cell death by changing the relative amount of Bc1-xL to Bim-EL.
On the previous day, uterine cervix cancer-derived HeLa cells were seeded over a 24-well plate at a concentration of 0.5×105 cells/well and cultured in a CO2 incubator at 37° C. On the next day, transfection was performed using Lipofectamine 2000 (Invitrogen Corp.) (trademark). To 0.3 μg of pENTR/H1/TO-shRNA-Box C/D-Bc1-xL, 0.2 μg of pBc1-xL, 0.2 μg of pBimEL, and 0.2 μg of pcDNA3.1-AsRed2-L7Ae were added and mixed with a medium, and 1.25 μl of Lipofectamine 2000 was added thereto. These DNA-lipid complexes were incubated at room temperature for 20 minutes and added dropwise to the medium for HeLa cells. Approximately 4 hours later, medium replacement was performed. For pcDNA3.1 (+) myc H is A vectors (Invitrogen Corp., control vector), pENTR/H1/TO-shRNA-Box C/D-mut Bc1-xL, pENTR/H1/TO-shRNA-Bc1-xL, and pENTR/H1/TO-shRNA-GFP mut (negative control), the same procedures were also performed.
24 hours after the transfection, the medium in each well was collected. Then, the cells were dissociated using 200 μl of Trypsin-EDTA and suspended by the addition of each medium collected in the previous step. The cell suspension was subjected to centrifugal sedimentation at 500× g at 4° C. for 3 minutes and washed with 300 μl of PBS. Then, to the cell pellet, a mixed solution of 3 μl of annexin V, Pacific Blue conjugate for flow cytometry (Invitrogen Corp.) and 50 μl of annexin-binding buffer (10 mM HEPES, 140 mM NaCl, 2.5 mM CaCl2, pH 7.4) was added. After tapping, the mixture was left standing at room temperature for 30 minutes for staining. Then, each sample was suspended by the addition of 200 μl of annexin-binding buffer. The cell suspension was transferred to a FACS tube and analyzed using FACSAria (BD). In this context, measurement was conducted for 30000 cells. For the analysis, first, cells emitting red fluorescence attributed to AsRed2-L7 were gated, and blue fluorescence intensity derived from Pacific Blue was measured for the cells within the gate using a filter at an excitation wavelength of 405 nm and a fluorescence wavelength of 430-470 nm. The ratio of the number of cells having this fluorescence intensity larger than the reference was measured. As the reference for determining cell death, phosphatidylserine, which is a lipid present in a manner specific for the outer membranes of dead cells, was stained with annexin V, Pacific Blue conjugate for flow cytometry (Invitrogen Corp.), and cells in which blue fluorescence intensity was larger than the upper limit of intensities of untreated cell samples stained in the same way were counted as dead cells.
As a result, the sample supplemented with the control vector (pcDNA3.1 (+) myc H is A vector) had a dead cell ratio of 8.3%, the sample supplemented with pENTR/H1/TO-shRNA-GFP mut (negative control) had a dead cell ratio of 10.1%, and the sample supplemented with pENTR/H1/TO-shRNA-Box C/D-Bc1-xL had a dead cell ratio of 13.4%. By contrast, the sample supplemented with pENTR/H1/TO-shRNA-Bc1-xL had a dead cell ratio of 34.5%, and the sample supplemented with pENTR/H1/TO-shRNA-Box C/D-mut Bc1-xL had a dead cell ratio of 42.5%. This experimental result and the Bc1-xL detection results shown in
According to a protein-responsive shRNA and an RNAi control system using an RNP motif according to the present invention, a sensor shRNA and a protein specifically binding to it can control RNAi and are thus useful in the construction of biosensors for quantifying the expression of intracellular marker proteins without destroying cells or artificial gene circuits capable of activating the translation of proteins of interest in response to the expression level of marker proteins. For example, the present invention produces significant effect that leads to the treatment of diseases such as cancer or Alzheimer's disease by activating apoptosis-inducing proteins in response to the expression of cancer marker proteins or as a basic technique for developing protein drugs.
Number | Date | Country | Kind |
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2008-312951 | Dec 2008 | JP | national |
Filing Document | Filing Date | Country | Kind | 371c Date |
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PCT/JP2009/070580 | 12/9/2009 | WO | 00 | 7/13/2011 |