The present invention relates to a protein involved in DNA replication as drug. The invention also relates to compounds inhibiting the expression or the activity of said protein.
Chromosomal DNA replication in eukaryotic cells is highly complicated and sophisticatedly regulated. Owing to its large size, a typical eukaryotic genome contains hundreds to tens of thousands of initiation sites called DNA replication origins where DNA synthesis takes place. Multiple initiation sites remove the constraint of a genome size because only a certain amount of DNA can be replicated from a single origin in a limited time. The activation of these multiple origins must be coordinated so that each segment of chromosomal DNA is precisely duplicated only once per cell cycle. Although DNA replication is a vital process for cell growth and its mechanism is highly conserved, recent studies also reveal significant diversity in origin structure, assembly of pre-replication complex (pre-RC) and regulation of replication initiation along evolutionary lines.
It is crucial to maintain genomic integrity in eukaryotic cells. During DNA replication, errors in pre-RC assembly often result in substantial changes in the amount of genetic material, which will cause cell death, or transform cells to become malignant tumors.
The first origin recognition complex (ORC) proteins to be identified were purified from cell extracts as a heterohexameric complex that specifically binds to origins of DNA replication and the subunits were named Orc1 through Orc6. Subsequently, orthologs of ORC1-ORC5 were identified in organisms as diverse as Drosophila melanogaster, Arabidopsis thaliana and Homo sapiens, strongly suggesting that these genes are likely to exist in all eukaryotes.
The ORC needs to be in an ATP-bound state so that it can interact with Cdc6p creating events that will produce the unwinding of the double stranded DNA which will promote the hydrolysis of the ATP by the ORC. Once the ORC is bound to the origin, the complex is retained in an ATP-bound state and the ATP hydrolysis is reserved for a downstream step in initiation. When the ORC binds to DNA at replication origin sites in an ATP-dependent manner it then serves as a scaffold for the assembly of other key initiation factors of the pre-replicative complex (pre-RC) which include Cdc6, Cdt1, and Mcm proteins.
Recently, mutations in genes encoding ORC1, ORC4, ORC6, CDT1, and CDC6 were identified in patients displaying Seckel syndrome (SS) and/or Meier-Gorlin syndrome (MGS) [Bicknell L S et al. (2011) Nat Genet 43: 356-359; Bicknell L S, et al. (2011) Nat Genet 43: 350-355; Guernsey D L, et al. (2011) Nat Genet 43: 360-364].
Seckel syndrome, Majewski osteodysplastic primordial dwarfism (MOPD) type II and Meier-Gorlin syndrome represent three disorders which share overlapping clinical features that include pronounced microcephaly, severe intrauterine growth retardation and post natal growth delay.
However, even if these mutations are associated with some of patients afflicted by these syndromes, some orphan individuals do not harbor any mutations or expression abnormality in the genes encoding ORC1, ORC4, ORC6, CDT1, and CDC6.
Therefore, there is a need to identify other genes in which mutations could be responsible of the syndromes developed by the above orphan individuals.
Another aim of the invention is to identify proteins that could be responsible of the above syndromes, or other syndrome linked to defects in unknown protein controlling DNA replication.
Still another aim of the invention is to provide a new efficient new medicine intended for the treatment of the above syndromes.
The invention relates to a composition comprising at least one of the following compounds:
The invention is based on the characterization by the inventors of a new protein that physically interacts with the ORC protein complex and that is involved in DNA replication.
By a purification process of the ORC protein complex, the inventors have identified a new ORC protein complex partner which has been identified to specifically interact with both ORC1 and LRWD1 proteins. The process for purifying the protein is described hereafter.
The ORC1 protein is a component of the origin recognition complex (ORC) that binds origins of replication. The DNA-binding of ORC1 is ATP-dependent.
The LRW1 protein is an associated component of the ORC required to recruit and stabilize the ORC complex to chromatin during G1 to establish pre-replication complex (preRC) and to heterochromatic sites in post-replicated cells. This protein binds a combination of DNA and histone methylation repressive marks on heterochromatin: it binds histone H3 and H4 trimethylation marks H3K9me3, H3K27me3 and H4K20me3 in a cooperative manner with DNA methylation.
The inventors have identified that the protein disclosed in databases as the RNF219 protein specifically interacts with only the above proteins (ORC1 and LRWD1) and is binding the ORC complex.
In view of the characterization of the interaction, RNF219 is now named: ORC Ubiquitin-ligase 1 or OBI1).
The human OBI1 protein consists of the amino acid sequence as set forth in SEQ ID NO: 1.
The composition according to the invention can therefore contain, as active substance, the OBI1 protein as set forth in SEQ ID NO: 1.
The invention also encompasses a protein derived from the protein as set forth in SEQ ID:1, said protein consisting of the amino acid sequence as set forth in SEQ ID NO: 1 and having at least one substitution and/or one deletion and/or one insertion of at least one nucleotide provided that said protein retains ubiquitin ligase activity and/or participates to DNA replication.
The invention encompasses also a composition as defined above, comprising as active substance a protein having at least 20% identity with SEQ ID NO: 1, in particular a protein having at least 20% identity with SEQ ID NO: 1 and containing the amino acid sequence SEQ ID NO: 28. SEQ ID NO: 28 represents the amino acid sequence of the zinc finger/ring finger of the OBI1 proteins.
Thus, in the invention, a protein having at least 20% identity with SEQ ID NO: 1 defines a proteins having 20% identity, 21% identity, 22% identity, 23% identity, 24% identity, 25% identity, 26% identity, 27% identity, 28% identity, 29% identity, 30% identity, 31% identity, 32% identity, 33% identity, 34% identity, 35% identity, 36% identity, 37% identity, 38% identity, 39% identity, 40% identity, 41% identity, 42% identity, 43% identity, 44% identity, 45% identity, 46% identity, 47% identity, 48% identity, 49% identity, 50% identity, 51% identity, 52% identity, 53% identity, 54% identity, 55% identity, 56% identity, 57% identity, 58% identity, 59% identity, 60% identity, 61% identity, 62% identity, 63% identity, 64% identity, 65% identity, 66% identity, 67% identity, 68% identity, 69% identity, 70% identity, 71% identity, 72% identity, 73% identity, 74% identity, 75% identity, 76% identity, 77% identity, 78% identity, 79% identity, 80% identity, 81% identity, 82% identity, 83% identity, 84% identity, 85% identity, 86% identity, 87% identity, 88% identity, 89% identity, 90% identity, 91% identity, 92% identity, 93% identity, 94% identity, 95% identity, 96% identity, 97% identity, 98% identity or 99% identity with SEQ ID NO: 1. Such proteins are, for instance, the proteins consisting of the amino acid sequence as set forth in SEQ ID NO: 2, SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6, SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12, SEQ ID NO: 13, SEQ ID NO: 14, SEQ ID NO: 15, SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, SEQ ID NO: 26 or SEQ ID NO: 27.
All these proteins represent the OBI1 proteins of different eukaryotic species. The above lists are not limitative, and the skilled person is able to determine any new Obi1 protein.
The invention also encompasses a composition comprising fragments of the above proteins, fragments retaining at least one of the function of the protein: i.e. said fragments retaining at least an oncogenic function, an ubiquitin ligase function or a dimerization function.
The advantageous fragments contained in the composition according to the invention are:
All the proteins and fragments as defined above can also be tagged with specific tags, in order to enhance and/or facilitate their purification. The tags can be located at the N-terminus part or at the C-terminus part of the proteins or fragments. In some advantageous embodiments, the proteins can be tagged at both their N- and C-terminus parts, such protein being advantageously tagged with two different tags.
The skilled person is able, with his common knowledge, to determine the most appropriated tags. The following list, which not intend to restrict the scope of the invention, represents the common tags that can be used: GFP, EGFP, YFP, CFP, dsRed, Myc tag, E tag, FLAG tag, Glu-Glu tag, GST tag, HA tag, His tag, in particular 6×HIS, HSV tag, luciferase, MBP, protein C tag, S tag, T7 tag, V5 tag, VSV-g tag, avidin/streptavidin/strep tag, thioredoxin, His-patch thioredoxin, 6-galactosidase, chloramphenicol acetyltransferase, cellulose binding domains (CBDs), chitin binding domain, staphylococcal protein A, streptococcal protein G, neo, hyg, pac, zeo, gpt, ble, dhfr, hpt and npt II.
It is also possible to use in the protein according to the invention nuclear sequences such as Nuclear Export Sequence (NES) or Nuclear Localization Signal (NLS), in order to specifically address respectively protein comprising them to the cytoplasm or the nucleus.
The invention also encompasses a composition comprising nucleic acid molecules coding for the proteins or the fragments as defined above.
In the invention the nucleic acid coding for the protein consisting of SEQ ID NO: 1 consists of the mRNA nucleic sequence as set forth in SEQ ID NO: 31.
The composition as defined above may also contain inhibitors of the expression or of the activity of the above mentioned protein.
In the invention salt(s), as used herein, means those salts of compounds of the invention that are safe and effective for use in mammals and that possess the desired biological activity. Pharmaceutically acceptable salts include salts of acidic or basic groups present in compounds of the invention. Pharmaceutically acceptable acid addition salts include, but are not limited to, hydrochloride, hydrobromide, hydroiodide, nitrate, sulfate, bisulfate, phosphate, acid phosphate, isonicotinate, acetate, lactate, salicylate, citrate, tartrate, oxalate, maleate, pantothenate, bitartrate, ascorbate, succinate, maleate, gentisinate, fumarate, gluconate, glucaronate, saccharate, formate, benzoate, glutamate, methanesulfonate, ethanesulfonate, benzensulfonate, p-toluenesulfonate, pamoate (i.e., 1,1′-methylene-bis-(2-hydroxy-3-naphthoate)), mesylate, besylate, tosylate and tartrate salts. Suitable base salts include, but are not limited to, aluminum, calcium, lithium, magnesium, potassium, sodium, zinc, and diethanolamine salts.
Advantageously, the invention relates to a composition as defined above, wherein said nucleic acid molecule comprises the nucleic acid sequence SEQ ID NO: 31, or a nucleic acid sequence having at least 20% identity, i.e. 20% identity, 21% identity, 22% identity, 23% identity, 24% identity, 25% identity, 26% identity, 27% identity, 28% identity, 29% identity, 30% identity, 31% identity, 32% identity, 33% identity, 34% identity, 35% identity, 36% identity, 37% identity, 38% identity, 39% identity, 40% identity, 41% identity, 42% identity, 43% identity, 44% identity, 45% identity, 46% identity, 47% identity, 48% identity, 49% identity, 50% identity, 51% identity, 52% identity, 53% identity, 54% identity, 55% identity, 56% identity, 57% identity, 58% identity, 59% identity, 60% identity, 61% identity, 62% identity, 63% identity, 64% identity, 65% identity, 66% identity, 67% identity, 68% identity, 69% identity, 70% identity, 71% identity, 72% identity, 73% identity, 74% identity, 75% identity, 76% identity, 77% identity, 78% identity, 79% identity, 80% identity, 81% identity, 82% identity, 83% identity, 84% identity, 85% identity, 86% identity, 87% identity, 88% identity, 89% identity, 90% identity, 91% identity, 92% identity, 93% identity, 94% identity, 95% identity, 96% identity, 97% identity, 98% identity or 99% identity, with the nucleic acid sequence SEQ ID NO: 31, provided that he protein coded by said nucleic acid sequences retains ubiquitin ligase activity, and/or participates to DNA replication.
In one another advantageous embodiment, the invention relates to a composition previously defined, wherein said nucleic acid molecule is contained in a vector, said vector comprising means allowing the expression of said nucleic acid molecule.
In the invention the vector is advantageously an expression vector which is a plasmid or virus designed for protein expression in cells. The vector is used to introduce a specific gene into a target cell, and can command the cell mechanism for protein synthesis to produce the protein encoded by the gene.
The vector is engineered to contain regulatory sequences that act as enhancer and promoter regions and lead to efficient transcription of the gene carried on the expression vector.
An expression vector have elements necessary for protein expression that include a strong promoter, the correct translation initiation sequence such as a ribosomal binding site and start codon, a strong termination codon, and a transcription termination sequence. There are differences in the machinery for protein synthesis between prokaryotes and eukaryotes, therefore the expression vectors must have the elements for expression that is appropriate for the chosen host. For example, prokaryotes expression vectors would have a Shine-Dalgarno sequence at its translation initiation site for the binding of ribosomes, while eukaryotes expression vectors contains the Kozak consensus sequence.
Vector may also comprise replication origin allowing the replication of the vector in bacteria. Furthermore, the vector as defined above may contain at least one selection marker allowing selection of transformed cells. These markers are well known in the art and the skilled person is able to determine which marker is more appropriate for a determined experiment.
In still another advantageous embodiment, the invention relates to a composition as previously defined wherein said compound inhibiting the expression of the protein consisting of an amino acid sequence as set forth in SEQ ID NO: 1, or the protein derived from the protein as set forth in SEQ ID:1 by substitution, deletion, or insertion of at least one nucleotide provided that this protein retains ubiquitin ligase activity and/or participate to DNA replication, in particular a protein having at least 20% identity with SEQ ID NO: 1 and containing the amino acid sequence SEQ ID NO: 28, as defined above, is chosen among a siRNA, miRNA, shRNA, RNA antisense, DNA antisense, antibodies and a fragment of the protein consisting of an amino acid sequence as set forth in SEQ ID NO: 1, said fragment comprising the amino acid sequence SEQ ID NO: 29, SEQ ID NO 30, SEQ ID NO: 59, SEQ ID NO: 60, SEQ ID NO: 61, SEQ ID NO: 62, SEQ ID NO: 63, SEQ ID NO: 100 or SEQ ID NO: 106.
siRNA, shRNA or miRNA according to the invention inhibit OBI1 gene expression by RNA interference mechanism.
RNA interference is a highly conserved biological mechanism inducing specific repression of genes by specifically destroying mRNA, or inhibition translation of said RNA.
In 1998, Fire et al [Fire et al., Nature. 1998 Feb. 19; 391(6669):806-11] demonstrated that a double-stranded is produced in cells by a Class III RNA endonuclease, the DICER complex, and small inhibiting double-stranded RNA (siRNA) of about 19 to 28 nucleotides are produced.
Incorporated to the enzymatic <<RNA-Induced Silencing Complex>> RISC complex, said siRNA are deshybridized and can therefore hybridize with the complementary sequence contained in mRNA. The “captured” mRNA is then destroyed, or its translation by ribosomal particles is inhibited.
Small hairpin RiboNucleic Acid—shRNA are double-stranded molecules comprising both the sense and the antisense strand of a siRNA, said sense and antisense strands being linked by a linker. These molecules form a hairpin, and the linker is eliminated to allow the liberation of a siRNA.
Micro RNA—miRNA are encoded by eukaryotic nuclear DNA and act as si- or mi-RNA.
The invention also relates to the composition as defined above, for its use as medicine. The invention further relates to the composition as defined above, for its use for the treatment or the prevention of a human or animal pathology linked to a dysfunction of the OBI1 gene or to the DNA replication.
In other words, the invention relates to a composition comprising at least one of the following compounds:
possibly in association with a pharmaceutically acceptable carrier, as defined above
for its use for the treatment or the prevention of a human or animal pathology linked to a dysfunction of the OBI1 gene as set forth in SEQ ID NO: 31 or the Obi1 protein as set forth in SEQ ID NO: 1, or the DNA replication.
The invention encompasses both:
The invention relates also to a method for treating human or animal pathology linked to a dysfunction of the OBI1 gene or linked to the DNA replication, said method comprising the administration of an effective amount, in a patient in a need thereof, of at least one of the following compounds:
Advantageously, the invention relates to the composition for its use according to the previous definition, wherein said pathology is a neoplastic disease or cancer, and wherein said composition comprises a compound inhibiting the expression of said nucleic acid molecule or the activity of said protein.
The compounds inhibiting the expression of the protein, i.e. the Obi1 protein, can be for instance the molecule inhibiting the expression by RNA interference. Such compounds are for instance those described hereafter.
The compounds inhibiting the activity of the protein, i.e. the Obi1 protein, are for instance compounds inhibiting the ubiquitin ligase activity of said protein.
Examples of such compounds are those discloses in Ceccarelli et al 2011 Cell 145:1075-87.
In one another advantageous embodiment, the invention relates to the composition for its use previously defined, wherein said pathology is a pathology linked to DNA replication is chosen among Meier-Gorlin syndrome, Seckel syndrome and Majewski osteodysplastic primordial dwarfism and wherein said composition comprises:
The invention also relates to a nucleic acid molecule inhibiting the expression of the OBI1 gene, as defined above by RNA interference, said a nucleic acid molecule comprising or consisting essentially of, or consisting of one of the following sequences:
The invention also relates to a composition, in particular for its use as defined above, comprising at least one of the nucleic acid molecules as defined above.
The complementary sequence of the nucleic acid molecule comprising or consisting of SEQ ID NO: 32 comprises or consists of the sequence SEQ ID NO: 40. The complementary sequence of the nucleic acid molecule comprising or consisting of SEQ ID NO: 33 comprises or consists of the sequence SEQ ID NO: 41. The complementary sequence of the nucleic acid molecule comprising or consisting of SEQ ID NO: 34 comprises or consists of the sequence SEQ ID NO: 42. The complementary sequence of the nucleic acid molecule comprising or consisting of SEQ ID NO: 35 comprises or consists of the sequence SEQ ID NO: 43. The complementary sequence of the nucleic acid molecule comprising or consisting of SEQ ID NO: 36 comprises or consists of the sequence SEQ ID NO: 44. The complementary sequence of the nucleic acid molecule comprising or consisting of SEQ ID NO: 37 comprises or consists of the sequence SEQ ID NO: 45. The complementary sequence of the nucleic acid molecule comprising or consisting of SEQ ID NO: 38 comprises or consists of the sequence SEQ ID NO: 46. The complementary sequence of the nucleic acid molecule comprising or consisting of SEQ ID NO: 39 comprises or consists of the sequence SEQ ID NO: 47.
Thus, most advantageous siRNA according to the invention are one of the following siRNA:
The above siRNA can also be modified by addition of compounds stabilizing siRNA structure.
For instance, the above siRNA may contain, in their 3′-end, a dinucleotide: a dithymidine (TT). Therefore, the siRNA according to the invention comprise one of the following sequences:
Thus, most advantageous siRNA according to the invention are one of the following siRNA:
In one another advantageous embodiment, the invention relates to a product used as mentioned above, wherein said shRNA comprises or consists of one of the following nucleic acid molecules:
The linker according to the invention can be chosen among the following linkers:
The compounds inhibiting the activity of the protein, i.e. the Obi1 protein, can be, for instance, the protein fragments interfering with the activity of the wild type Obi1 protein. Such fragments are for instance those as set forth in SEQ ID NO: 29, SEQ ID NO 30, SEQ ID NO: 59, SEQ ID NO: 60, SEQ ID NO: 61, SEQ ID NO: 62, SEQ ID NO: 63, SEQ ID NO: 100 or SEQ ID NO: 106, in particular the fragments as set forth in SEQ ID NO: 29, SEQ ID NO: 61, SEQ ID NO: 100 and SEQ ID NO: 106.
The invention also relates to an inhibitor of the activity of the protein consisting of an amino acid sequence as set forth in SEQ ID NO: 1, or a protein derived from the protein as set forth in SEQ ID:1 by substitution, deletion, or insertion of at least one nucleotide provided that said protein retains ubiquitin ligase activity and/or participates to DNA replication, as defined above, characterized in that it comprises the amino acid sequence: SEQ ID NO: 29, SEQ ID NO 30, SEQ ID NO: 59, SEQ ID NO: 60, SEQ ID NO: 61, SEQ ID NO: 62, SEQ ID NO: 63, SEQ ID NO: 100 or SEQ ID NO: 106.
The above fragments may be used as purified proteins, in particular in association with an appropriate salt, or in a form of nucleic acid coding said fragment, possibly contained in a vector (viral vector), possibly in the vector comprising a Myc tag, and possibly derived from the vector as set forth in SEQ ID NO: 107.
These proteins, or fragments, and their nucleic acids are artificial, non naturally occurring, or purified from their natural context.
The invention further relates to the use of the protein consisting of an amino acid sequence as set forth in SEQ ID NO: 1, or protein derived from the protein as set forth in SEQ ID:1 by substitution, deletion, or insertion of at least one nucleotide provided that said protein retains ubiquitin ligase activity and/or participates to DNA replication, as defined above, or a fragment thereof as defined above as Lys6 ubiquitine ligase enzyme.
The invention also relates to a method for ubiquitinate at least one protein, in particular ORC3 and ORC5 subunits of the ORC complex, comprising a step of contacting said protein with the protein consisting of an amino acid sequence as set forth in SEQ ID NO: 1, protein derived from the protein as set forth in SEQ ID:1 by substitution, deletion, or insertion of at least one nucleotide provided that said protein retains ubiquitin ligase activity and/or participates to DNA replication, or a fragment thereof as defined above,
said protein comprising a chain of Lys6-linked poly ubiquitin.
The RING ligases that have been characterized to date yield different patterns of substrate ubiquitination.
RING domains recruit E2 enzymes that are thioesterified with ubiquitin and also activate E2 to discharge its ubiquitin cargo to a substrate.
A number of RING ligases primarily monoubiquitinate or oligoubiquitinate their substrates. Ubiquitination may terminate after the transfer of only one or a few ubiquitins because the substrate simply falls off the E3 before the reaction can proceed further. However, oligoubiquitination is specified by an internal ubiquitin-binding domain that caps the growing chain and prevents its further extension. Yet other E3-E2 pairs transfer multiple ubiquitins to substrate, but in the form of several monoubiquitins rather than a polyubiquitin chain.
Multiple monoubiquitination can directly promote degradation of cyclin B in vitro but most often probably does not function as a proteasome-targeting signal in vivo, as exemplified by modification and lysosomal targeting of the EGF receptor by c-Cbl. Other RING-E2 complexes transfer multiple ubiquitins to substrate preferentially in the form of a polyubiquitin chain.
RING-E2 complexes can assemble chains linked exclusively via the Lys6, Lys48, and Lys63 residues of ubiquitin. Ultimately, all seven lysine residues of ubiquitin (Lys6, Lys11, Lys27, Lys29, Lys33, Lys48, Lys63) can form chain linkages in vivo. Thus, the number of topological isomers is potentially huge if chains of mixed linkage are produced.
These modifications have a range of biological effects, from proteasome-dependent proteolysis (Lys48- and Lys11-linked polyubiquitin) to posttranslational control of protein function, structure, assembly, and/or localization (Lys63 and other linkages). The inventors have demonstrated that OBI1 protein is an E3 ubiquitin ligase that essentially forms Lys6 polyubiquitin chains (see example section).
The invention also relates to the use of an inhibitor of the protein consisting of an amino acid sequence as set forth in SEQ ID NO: 1, protein derived from the protein as set forth in SEQ ID:1 by substitution, deletion, or insertion of at least one nucleotide provided that said protein retains ubiquitin ligase activity and/or participates to DNA replication, as defined above, for inhibiting cell proliferation.
The inventors have demonstrated that OBI1 gene is an oncogene, as set forth in the example section.
Therefore, the inventors propose, and have tested, inhibitors of the expression, and/or activity of OBI1 in order to abolish its oncogenic function and in order to inhibit deregulated cell proliferation.
The invention also encompasses a composition comprising at least one inhibitor of the protein consisting of an amino acid sequence as set forth in SEQ ID NO: 1, or protein derived from the protein as set forth in SEQ ID:1 by substitution, deletion, or insertion of at least one nucleotide provided that said protein retains ubiquitin ligase activity and/or participates to DNA replication, as defined above, for its use for treating cancer. The invention relates also to a method for treating cancer comprising the administration of an effective amount, to a patient in a need thereof, of at least one inhibitor of the protein consisting of an amino acid sequence as set forth in SEQ ID NO: 1, or protein derived from the protein as set forth in SEQ ID:1 by substitution, deletion, or insertion of at least one nucleotide provided that said protein retains ubiquitin ligase activity and/or participates to DNA replication, as defined above.
The invention further relate to a process for purifying a protein consisting of the amino acid sequence SEQ ID NO: 1, or protein derived from the protein as set forth in SEQ ID:1 by substitution, deletion, or insertion of at least one nucleotide provided that said protein retains ubiquitin ligase activity and/or participates to DNA replication, as defined above, said process comprising:
In the invention, the ORC1 and LRWD1 proteins consist respectively of the amino acid sequence as set forth in SEQ ID NO: 57 and 58.
The invention further relate to a process for purifying a protein consisting of the amino acid sequence SEQ ID NO: 1, or protein derived from the protein as set forth in SEQ ID:1 by substitution, deletion, or insertion of at least one nucleotide provided that said protein retains ubiquitin ligase activity and/or participates to DNA replication, as defined above, said process comprising the steps of:
In one other advantageous embodiment, the invention relates to a process for purifying a protein consisting of the amino acid sequence SEQ ID NO: 1, or protein derived from the protein as set forth in SEQ ID:1 by substitution, deletion, or insertion of at least one nucleotide provided that said protein retains ubiquitin ligase activity and/or participates to DNA replication, said process comprising the steps of:
The above method is well known in the art as TAP-TAG purification process as discloses in Puig et al. METHODS 24, 218-229 (2001).
Tandem affinity purification (TAP) is a technique for studying protein-protein interactions. It involves creating a fusion protein with a designed piece, the TAP tag, on the end.
In the original version of the technique, the protein of interest with the TAP tag first binds to beads coated with IgG, the TAP tag is then broken apart by an enzyme, and finally a different part of the TAP tag binds reversibly to beads of a different type. After the protein of interest has been washed through two affinity columns, it can be examined for binding partners.
The original TAP method involves the fusion of the TAP tag to the C-terminus of the protein under study. The TAP tag consists of calmodulin binding peptide (CBP) from the N-terminal, followed by tobacco etch virus protease (TEV protease) cleavage site and Protein A, which binds tightly to IgG. The relative order of the modules of the tag is important because Protein A needs to be at the extreme end of the fusion protein so that the entire complex can be retrieved using an IgG matrix.
Once the fusion protein is translated within the host, the new protein at one end of the fusion protein would be able to interact with other proteins. Subsequently, the fusion protein is retrieved from the host by breaking the cells and retrieving the fusion protein through affinity selection, together with the other constituents attached to the new protein, by means of an IgG matrix.
After washing, TEV protease is introduced to elute the bound material at the TEV protease cleavage site. This eluate is then incubated with calmodulin-coated beads in the presence of calcium. This second affinity step is required to remove the TEV protease as well as traces of contaminants remaining after the first affinity step.[2] After washing, the eluate is then released with ethylene glycol tetraacetic acid (EGTA).
The native elution, consisting of the new protein and its interacting protein partners as well as CBP, can now be analyzed by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) or be identified by mass spectrometry.
The invention further relates to an isolated purified protein complex comprising the protein consisting of the amino acid sequence as set forth in SEQ ID NO: 1, or protein derived from the protein as set forth in SEQ ID:1 by substitution, deletion, or insertion of at least one nucleotide provided that said protein retains ubiquitin ligase activity and/or participates to DNA replication, as defined above, and the ORC1 protein or the LRWD1 protein, or both.
In the invention the ORC1 protein consists of the amino acid sequence SEQ ID NO: 57, and the LRWD1 protein consists of the amino acid sequence SEQ ID NO: 58.
The complex as defined above comprises, or consists essentially, or consists of
This complex may contain nucleic acid molecules.
The invention further relates to a process for identifying compounds destabilizing the complex defined above, said method comprising the following step:
According to the above described method, it is possible to screen compounds able to destabilize the above complex, i.e. able to inhibit the interaction between Obi1 and ORC1 or between OBI1 and LRWD1.
The process as defined above is such that, if the purification of OBI1 is not effective, then the tested compound has destabilized the complex, and if the purification of OBI1 is effective, thus the tested compound is not able to destabilize the complex.
One advantageous embodiment of this process is to use fluorescent ORC proteins and OBI1 protein. Such fluorescent proteins are obtained by adding a fluorescent tag. In this embodiment, the fluorescent proteins are able to carry out FRET (Fluorescent rescue energy transfer), such that the emitting wavelength of one of the fluorescent protein corresponds to the absorption wavelength of the other protein.
Therefore, when proteins are close, the complex is detected by exposing cells with a wavelength corresponding to the absorption wavelength of the first fluorescent molecule and by detecting the light with a filter corresponding to the emission wavelength of the second molecule.
If the complex is destabilized, it is therefore impossible to detect the light with a filter corresponding to the emission wavelength of the second molecule, since no FRET is able.
The invention also relates to a method for diagnosing, advantageously in vitro or ex vivo, Meier-Gorlin syndrome, Seckel syndrome and Majewski osteodysplastic primordial dwarfism, comprising a step of identifying the sequence of the Obi1 gene in cells originating from an individual, and a step of comparing said sequence with a reference sequence as set forth in SEQ ID NO: 97.
As demonstrated in Example 12, the inventors have identified in a patient afflicted by Meier-Gorlin syndrome a mutation (a deletion) which leads to a frameshift. The mutation therefore leads to the expression of a truncated protein.
Thus, by identifying the sequence of the Obi1 gene, by sequencing said gene, it is possible to determine if an individual is liable to be afflicted by Meier-Gorlin syndrome. From cells form an individual suspected to be afflicted by Meier-Gorlin syndrome, it is possible to specifically amplify, by PCR, the Obi1 gene, in particular the open reading frame (ORF) of said gene, and thus to sequence this ORF. By comparison with a reference sequence, in particular the sequence as set forth in SEQ ID NO: 97, it is possible to determine if a mutation has occurred, and if said mutation affect the biological function of the resulting protein.
It is also possible to diagnose Meier-Golin syndrome, Seckel syndrome and Majewski osteodysplastic primordial dwarfism, by measuring, possibly in vitro or ex vivo, in cell from an individual suspected to be afflicted by said syndromes, the total activity of the Obi1 protein consisting of the amino acids sequence SEQ ID NO: 1.
If the total Obi1 activity is less that the Obi1 activity of a control cell (originating from healthy individual), preferably at least 1.5× lower than the activity of the control cell, thus the individual is probably afflicted by said syndrome.
The total activity can be measured by determining the Lys6 ubiquitine ligase activity of the proteins co-immuno precipitating with ORC1.
In view of the above description, the skilled person may easily specifically identify such a total Obi1 activity in cells.
The invention advantageously relates to a method for diagnosing Meier-Gorlin syndrome, Seckel syndrome and Majewski osteodysplastic primordial dwarfism, in an individual suspected to have or suspected to further develop said syndrome, said method comprising a step of sequencing the Obi1 cDNA to obtain its sequence, and comparing the obtained sequence with a reference sequence, and in particular with SEQ ID NO: 97.
The skilled person is able to easily determine the above mentioned sequence.
The invention will be better explained in view of the following examples and the following figures.
U20S, HeLa S3, NIH 3T3 and Platinum-E (Cell Biolabs) cells were grown in DMEM (Invitrogen) supplemented with 10% Foetal Bovine Serum (FBS), 2 mM glutamine and antibiotics. Cells were transfected using the Lipofectamine reagent (Invitrogen) as specified by the manufacturer. For TAP-TAG experiments, HeLa S3 cells stably expressing baits were generated by retroviral transduction. For this, viral particles were generated using Platinum-E ecotropic packaging cell line transiently transfected with the retroviral constructs. In parallel, HeLa S3 cells were transiently transfected with mouse Cationic Aminoacid Transporter 1 to render them susceptible to infection by ecotropic retroviruses. 48 hours after transfection, S3 cells were incubated with viral supernatant in presence of polybrene (10 um/mL, Sigma Aldrich) for 24 hours. 48 hours later, transduced cells express human IL2 receptor alpha chain which allows selection using mouse anti-IL2Ra antibody (Upstate Biotechnology) coated magnetic beads as specified by the manufacturer (Dynabeads M-450 Epoxy, Invitrogen). Knockdown experiments were done using a pool of 4 siRNAs (Smartpool, Dharmacon) targeting human Obi1 transfected using Interferin reagent (PolyPlus Transfection) as specified by the manufacturer. 10 nM siRNA was added to the cells.
Anti-Flag M2 [# F1804; 1/1000], anti-Actin [# A5441; 1/5000] and anti-PCNA [# WH0005111M2; 1/2500] monoclonal antibodies were from Sigma. The anti-Myc 9B11 monoclonal antibody [#2276S; 1/1000] was from Cell Signaling Technologies. The polyclonal antibodies against HA [# sc-805; 1/100], Obi1/RNF219 [# sc-84039; 1/100] and ORC4 [# sc-20634; 1/100] were from Santa-Cruz BioTechnologies. The anti-ORC2 antibody [ 1/1000] was described previously (Cayrou et al. (2011) Genome Res 21:1438-49.)
For TAP-TAG experiments, human ORC1, ORC2 and LRWD1 were amplified by PCR using cloned cDNA as template with the following primers:
These primers introduced a Not I restriction enzyme site at both end of the cDNA. Using Pfu polymerase (Promega) as specified by the manufacturer: The following PCR conditions were:
4) 2 min/kb extension time at 73° C.
5) repeat step 2-4 25 times
PCR products were purified (Qiaquick, Qiagen) and digested with NotI. The DNA fragments were subcloned at the Not I site of pOZ-FH-C to produce a protein having an inframe C-Terminal Flag-HA tag. Restriction digestion and sequencing analysis allowed us to screen for the proper construction. For co-immunoprecipitation and ubiquitination studies, a vector expressing an N-Terminal Flag tag was constructed. The pCS2 vector was digested with BamHI/EcoRI fragment, which removes the Myc6 tag and ligated with the following annealed oligos:
This yields pCS2-Flag. Then, ORC1-6 were amplified by PCR using the cloned cDNA as template with the following template:
These primers introduced the indicated sites at both end of the cDNA. Using Pfu polymerase (Promega) as specified by the manufacturer: The following PCR conditions were:
4) 2 min/kb extension time et 73° C.
5) repeat step 2-4 25 times
PCR products were purified (Qiaquick, Qiagen) and digested with the appropriate restriction enzymes. The DNA fragments were subcloned at the relevant site in pCS2-FLAG vector. Restriction digestion and sequencing analysis allowed us to screen for the proper construction. To construct human Myc6-tagged Obi1 WT expression vectors, we amplified by PCR using the cloned cDNA as template with the following template:
For Obi1 ΔRING, the following primer were used:
For Obi1 ΔCTD/OBD, the following primers were used:
For Obi1 CC, the following primers were used:
For Obi1 CTD/OBD, the following primers were used:
These primers introduced the indicated sites at both end of the cDNA. Using Pfu polymerase (Promega) as specified by the manufacturer: The following PCR conditions were:
4) 2 min/kb extension time et 73° C.
5) repeat step 2-4 25 times
PCR products were purified (Qiaquick, Qiagen) and digested with NcoI/XbaI. The DNA fragments were subcloned at the relevant site in pCS2.
To construct ObiΔCC, the RING domain of Obi1 was amplified with the following primer:
and cloned at the NcoI of pCS2-Obi1 CTD/OBD. Restriction digestion and sequencing analysis allowed us to screen for the proper construction. To construct Xenopus Myc6-tagged Obi1 WT expression vectors, we amplified by PCR using the cloned cDNA as template with the following template:
PCR products were purified (Qiaquick, Qiagen) and digested with EcoRI/XhoI. The DNA fragments were subcloned at the relevant site in pCS2. HA-tagged ubiquitin WT and K mutants are described (Sobhian et al. (2007) Science 316:1198-202.). For re-replication experiments, human WT Cdt1 with an C-Terminal HA-tag was generated.
First, pcDNA3 (Invitrogen) was digested with EcoRI/XbaI and the following annealed oligos were cloned:
To yield pcDNA3-HACT. Then, human WT Cdt1 was amplified by PCR using cloned cDNA as template with the following primers:
PCR products were purified (Qiaquick, Qiagen) and digested with HindIII/EcoRI. The DNA fragments were subcloned at the relevant site in pcDNA3-HACT. pEGFP-C2 (Clontech) was used an EGFP expression vector. In chromatin fractioning experiments, Flag-tagged human MCM2 and MCM5 have been described (Tardat et al (2010) Nat Cell Biol 12:1086-93.)
U20S cells were co-transfected with the tested constructs and an expression plasmid coding for EGFP. 60-72 h post-transfection, cells were trypsinized and fixed in 1% paraformaldehyde in PBS at RT for 15 min. Washed cells were fixed again in 70% ethanol in PBS and stored at −20° C. overnight. Cells were spun at 2000 rpm for 10 min, washed in PBS and treated with 50 μg/mL RNAse A. DNA was stained with 25 μg/mL propidium iodide. Cells were analysed with a FACSCalibur flow cytometer using the CellQuestPro software.
For cell lysis, immunoprecipitation and western blotting were performed following standard methods. Briefly, cells were lysed in TK300 lysis buffer (20 mM Tris-HCl pH 7.9; 300 mM KCl, 5 mM MgCl2, 10% glycerol; 0.5% NP-40 plus protease inhibitors cocktail) on ice for 30 min. The protein concentration of the clarified lysates was estimated using the BCA method (Pierce). For immunoprecipitation experiments, equivalent amounts of protein samples were incubated at 4° C. with anti-Flag coupled agarose beads (Sigma Aldrich) for 4 h. After extensive washing with TK300 lysis buffer, bound proteins were eluted in boiling Laemmli buffer. Samples were runs on pre-cast gradient gel (NuPage Novex, Invitrogen and Mini-PROTEAN TGX, Biorad) and transferred to nitrocellulose membrane. Western blot were revealed using ECL prime (Amersham).
U20S cells were co-transfected with Flag-tagged ORC subunits along with HA-ubiquitin (WT or K only mutants). In some cases, Obi1 (WT or mutants) was co-transfected. In other cases, endogenous Obi1 expression was silenced by treated the cells with Obi1 siRNAs 24 hours before plasmid transfection. 48 hours after plasmid transfection, cells were lysed in Triton X-100 lysis buffer (50 mM Tris-HCl pH=7.4; 100 mM NaCl; 50 mM NaF; 5 mM EDTA; 40 mM β-glycero-phosphate; 1% Triton X-100 plus protease inhibitors cocktail) supplemented with 10 mM N-ethyl maleimide (NEM, Sigma) to inhibits deubiquitinating enzymes. Cell lysates (750 μg protein) were then incubated for 2 h at 4° C. with anti-Flag coupled agarose beads (Sigma Aldrich). The bound proteins were washed 5 times in lysis buffer and resolved on gradient gels. Ubiquitin-containing conjugates were detected by immunoblotting with anti-HA antibody.
Chromatin and soluble fractions were obtained using the CSK procedure. Briefly, cells were lysed in CSK buffer (10 mM PIPES pH=6.8; 100 mM NaCl; 300 mM sucrose; 1 mM MgCl2; 0.5 mM DTT; 0.2% Triton X-100; 1 mM ATP plus protease inhibitor cocktail) on ice for 10 min. Insoluble material was pelleted (3000 rpm, 4° C., 3 min). Supernatants (soluble fraction) were kept, while pellets were extracted a second time in CSK buffer. The final pellets (chromatin fraction) were solubilized in Laemmli buffer.
NIH 3T3 cells stably expressing human Obi1 or the empty vector were plated in duplicate in 60 mm plates at equivalent density. Confluent cells were cultured for 2-3 weeks and the culture medium was changed every 2-3 days. Foci were stained with crystal violet dye.
105 cells of NIH 3T3 cells stably expressing human Obi1 or the empty vector were mixed with medium supplemented with 0.4% noble agarose (sigma) and placed on top of the 1% agarose layer. 1 mL medium was added to the solidified layer and changed every 2-3 days. After 3-4 weeks, colonies were counted in 10 randomly selected fields using a phase contrast microscope.
Hela S3 cells (40*150 mm confluent dishes) were trypsinized to obtain a homogenous cell suspension. After a wash in PBS, cells were lyzed in a hypotonic buffer (HB buffer: 10 mM Tris pH 7.9; 1.5 mM MgCl2; 10 mM KCl; 1 mM DTT; 10 mM PMSF). Briefly, cells were washed once in ice cold HB buffer (10 times the cell pellet volume (CPV). The pelleted cell pellet was then resuspended in 2 times CPV of HB buffer. Cells were incubated on ice for 10-15 min. Swollen cells are transferred to a dounce homogenizer and cells were lyzed by 15 stroke using the tight pistol. The nuclei are pelleted by centrifugation. The supernatant is discarded and the nuclei are resuspended in 0.5 nuclear pellet volume (NPV) of Low Salt (LS) buffer (20 mM Tris pH 7.9; 1.5 mM MgCl2; 0.2 mM EDTA; 20 mM KCl; 1 mM DTT; 10 mM PMSF). Whilst gently vortexing the tube, add 0.5×NPV of High Salt (HS) buffer (20 mM Tris pH 7.9; 1.5 mM MgCl2; 0.2 mM EDTA; 1200 mM KCl; 1 mM DTT; 10 mM PMSF) drop by drop. After a 30 min incubation with agitation in the cold room, the Dignam nuclear extracts are clarified by centrifugation and freeze in liquid nitrogen. The extracts were kept at −80 C
All procedures were done at 4 C and on ice. Thaw Dignam extract on ice for 30-45 min. Spin (13 000 rpm, 20 min) to clarify the extract. A typical experiment involves ˜10 mL of extract. We first performed the Flag IP. We use 1% volume/volume of anti-Flag coupled agarose beads (Sigma, ˜100 μL). Beads were washed to diminish background binding: ¼ volume beads of 0.1 M Glycine pH=2.2 was added to the beads and incubate for 3 min at room temperature. ½ volume beads of Tris 1M pH=7.9 was added. The beads were washed twice with 1 mL of HA-IP Buffer (150 mM KCl; 20 mM Tris pH 7.5 0.05% NP40; 0.1% Tween; 10% Glycerol; 5 mM MgCl2; 1 mM DTT and 10 mM PMSF). After the last centrifugation, beads were resuspended in HA-IP Buffer (1 vol of Beads). Extracts were incubated with Flag beads for 4 h with agitation at 4 C. Beads were pelleted (3 min at 3000 rpm 4° C.). Beads were washed 5 times with HA IP Buffer: Beads are pelleted (3K 3 min 4° C.) and the supernatant discarded. Complexes were eluted from the beads by incubating in 3 beads volume of HA IP Buffer supplemented with Flag peptide (200 μg/mL, Sigma) for 1 hour at 4 C with agitation. The supernatant was kept on ice and a second elution was conducted. The eluates were pooled and subjected to an anti-HA immunoprecipitation. Before, anti-HA coupled agarose beads (SantaCruz Biotechnology) were washed with glycine buffer as described above. 10 μL of beads was used per IP. Flag eluates were incubated with anti-HA beads for 2 hours at 4 C with agitation. Beads were pelleted (3 min at 3000 rpm 4° C.). Beads were washed 5 times with HA IP Buffer: Beads are pelleted (3K 3 min 4° C.) and the supernatant discarded. Complexes were eluted from the beads by incubating in 3 beads volume of HA IP Buffer supplemented with HA peptide (400 μg/mL, Roche) for 1 hour at 4 C with agitation. The supernatant was keep on ice and a second elution was conducted. HA eluates were clarified on a filter column (Pierce Spin Cups Cellulose Acetate Filter ThermoFisher): columns were rinsed with 400 μl of HA IP buffer and spun for 1 min at 7000 rpm at 4° C. The supernatant was discarded and eluates were apply to the column. After spinning, the flow-through was collected and denatured in lammeli buffer. 25% of the samples were run in precast NuPage gradient gel and stained by silver nitrate (SilverQuest, Invitrogen) as specified by the manufacturer. 75% of samples were run on precast gel and stained with colloidal blue staining kit (Invitrogen) as specified by the manufacturer.
Bands on colloidal blue stained gels were excised, reduced with DTT and alkylated with lodoacetamine (IAA) using standard procedure. Bands were then subjected to trypsin (Promega) digestion. Extracted peptides were collected and analysed using a nanoESI LTQ_XL Orbitrap mass spectrometer (Thermo Fisher Scientific) coupled to an Ultimate 3000 HPLC (Dionex). A gradient of 0-40% B for 30 min and 80% B for 15 min (A=0.1% formic acid, 2% acetonitrile in water; B=0.1% formic acid in acetonitrile) at 300 nl/min was used to elute peptides from the capillary (0.075 mm×150 mm) reverse-phase column (Pepmap®, Dionex). Nano-ESI was performed with a spray voltage of 2.4 kV, heated capillary temperature of 200° C., and tube lens voltage of 140 V. A cycle of one full-scan mass spectrum (400-1600 m/z) at a resolution of 30000, followed by five data-dependent MS/MS spectra was repeated continuously throughout the nanoLC separation. All MS/MS spectra were recorded using normalized collision energy and an isolation window of 2 m/z. Data were acquired using the Xcalibur software (v 2.0.7, Thermo Fisher Scientific). Data analysis was performed using MaxQuant 1.3.0.5 and standard parameters against the CPS_HUMAN database (November 2012). FDR was set at 1%.
Identification of the interaction partners of a particular protein became a valuable way to gain insight into the physiological role of the protein.
The most widely used system to identify intermolecular interactive partners of a particular protein of interest is the yeast two-hybrid system. However, given that this system is designed to detect mostly binary interactions, it is not suitable for investigating the intermolecular interaction partners of a protein if the latter is a component of a multimeric protein complex.
For identification of intermolecular interaction partners, purification of the native protein complexes from the cells would be the best method. This would provide information on how the endogenous protein interacts with intermolecular interaction partners.
However, in general, purification of native complexes is technically difficult and time-consuming, especially when the protein of interest is scarce. These limitations can be addressed with epitope tagging. It has been shown that stably expressed exogenous proteins with epitope tags are integrated into the complexes when the complex is synthesized de novo. Such a protein complex can be purified rapidly by immunoprecipitation with antibodies against epitopes.
The inventors took advantage of the epitope-tagging technique to develop a standardized approach to purifying multimeric protein complexes from mammalian cells. We put two different epitope tags tandemly (i.e., FLAG and HA) on the C terminus of the proteins of interest. For rapid generation of cell lines that express the epitope-tagged proteins of interest, the inventors used retroviral transduction. The cells are sorted magnetically after transduction. Once stably transduced cell lines are established, the protein complex can be purified from cells in less than 24 h.
The above steps are represented in
Results of TAP-TAG assays are reproduced on
These data demonstrates that Obi1/RFN219 interacts specifically with ORC1 and LRWD1, but is undetectable for ORC2.
In order to validate the TAP-TAG interaction, the inventors have tested the Obi1-ORC1 interaction in vitro by co-immunoprecipitation.
Results are shown in
As shown, immunoprecipitation of ORC1 co-immunoprecipitate Obi1 protein, confirming the interaction observed in TAP-TAG assay.
Further, to determine Obi1 domains involved in ORC1/Obi1 interaction, the inventors have constructed Obi1 deletion fragments of Obi1 and evaluated their ability to interact with ORC1. Constructions are shown in
To further identify biochemical properties of Obi1, the inventors have evaluated its ability to self-associate.
The deletion mutants described in
Results are shown in
It is to be noticed that all constructs having the Coiled-coil region can dimerize with WT Obi1.
Since ORC1 participate to DNA replication, the inventors have evaluated Obi1 function during DNA replication.
In
Since Obi1 participate to DNA replication by inducing re-replication of DNA, the inventors have investigated the oncogenic potential of Obi1.
These data demonstrate that Obi1 behaves like a proto-oncogene.
Since Obi1 protein contains a RING domain, the inventors have evaluated its participation in protein ubiquitination process.
The inventors have first evaluated the ubiquitination of ORCs protein in vitro in presence of Obi1 protein.
In a second time, the inventors have demonstrated that ubiquitination is essentially carried out via Ubiquitin Lys6. Indeed, as shown in
These data demonstrate that Obi1 is a K6 polyubiquitin ligase.
In vitro experiments, shown in
The inventors have tested if the poly-ubiquitin ligase activity of human Obi1 protein is conserved.
As shown in
These results demonstrate that the activity of Obi1 on ORC polyubiquitylation is conserved toward species.
To determine the importance of the Obi1 in poly-ubiquitination of ORC, the inventors have invalidated Obi1 gene by RNA interference.
Obi1 is thus the major ORC ubiquitin ligase in vivo.
To further evaluate the function of Obi1, the inventors have evaluated the proliferation of cells in which Obi1 expression has been inhibited by siRNAs.
Moreover,
In order to determine where Obi1 protein is expressed, the inventors have transiently expressed a tagged Obi1 protein in U20S cells. Vectors comprising nucleic acid allowing the expression of a Myc-tagged Obi1 protein, or an empty vector were transiently transfected in U20S cells 48 hours post-transfection, cells were fixed in 2% paraformaldehyde/PBS, permabilized and stain using an anti-Myc mouse monoclonal antibody followed by a anti-Mouse FITC coupled antibody. Nuclei were stained using Hoescht (10 mg/ml). (
To further understand the underlying activity of Obi1 protein during cell cycle, the inventors have developed a mutant form of Obi1 protein. Based on their findings, the inventors know that Obi1 is an homodimeric protein predominantly localized in the nucleus, where it can interact with its substrate, the ORC complex.
The inventors have developed a mutant form of Obi1 lacking the CTD/OBD domain and including a nuclear export sequence (NES), allowing the exit of the protein comprising it from the nucleus.
By fusion of the Obi1 dimerization domain (Coiled-coil) with a Nuclear Export Sequence (NES, derived from PKI), the inventors hypothesised to drive endogenous Obi1 out of the nucleus and away from its substrate. In addition, the heterodimer NES-Obi1(1-280)/Obi1 WT is inactive as it is also unable to bind to the ORC Complex. The nucleic acid molecule coding for said NES-Obi1(1-280) protein consists of the sequence as set forth in SEQ ID NO: 105. The NES-Obi1(1-280) protein consists of the amino acid sequence as set forth in SEQ ID NO: 106.
To obtain the Obi1 inhibitor Myc-NES-Obi1(1-280), a vector harboring the nuclear export sequence (NES) of the Protein Kinase A Inhibitor (PKI) was first constructed. For this, the pCS2+MT (SEQ ID NO: 107) vector was digested with NcoI/EcoRI, which removes the 6th Myc tag and ligated with the following annealed oligos:
This yields pCS2+MT-NES which expressed Myc-NES tagged proteins. Note that the ligated NcoI site is inactivated and a functional NcoI is reintroducted 3′ of the NES sequence. Then, Obi1 ΔCTD/OBD (which is the same as Obi1(1-280)) was amplified by PCR using the cloned Obi1 cDNA as template with the following template:
These primers introduced NcoI/XbaI sites at both end of the cDNA. Using Pfu polymerase (Promega) as specified by the manufacturer: The following PCR conditions were:
4) 2 min/kb extension time at 73° C.
5) repeat step 2-4 25 times
PCR products were purified (Qiaquick, Qiagen) and digested with NcoI/XbaI. The DNA fragments were subcloned into NcoI/XbaI digested pCS2+MT-NES. Restriction digestion and sequencing analysis allowed us to screen for the proper construction.
The inventors first assessed the subcellular localisation of the NES-Obi1(1-280) mutant form. U20S cells were transiently transfected with plasmids coding for Myc-tagged NES-Obi1(1-280). 24 hours post-transfection, cells were fixed in 2% paraformaldehyde/PBS, permabilized and stain using an anti-Myc mouse monoclonal antibody followed by a anti-Mouse FITC coupled antibody. Nuclei were stain using Hoescht (10 mg/ml) (
Thus, to confirm that NES-Obi1(1-280) protein still associate with endogenous Obi1 protein, the inventors have tested the interaction between the two proteins. U20S cells were transiently transfected with plasmids coding for Myc-tagged-NES-Obi1(1-280) along with Flag-Obi1 WT. 24 hours post-transfection, cells were lyzed and the soluble fraction (linput,
Further, the inventors have evaluated the cellular localisation of WT-Obi1 protein when co-expressed with NES-Obi1(1-280). U20S cells were transiently transfected with plasmids coding for Flag-tagged WT Obi1 along with Myc-tagged NES-Obi1(1-280) or the empty vector. 24 hours post-transfection, cells were fixed in 2% paraformaldehyde/PBS, permabilized and stain using an anti-Flag mouse monoclonal antibody followed by a anti-Mouse FITC coupled antibody. Nuclei were stain using Hoescht (10 mg/ml). The position of the transfected nuclei is indicated by a white arrow. The localization of the ectopic protein was scored on at least 100 cells based on the nuclear:cytoplasm distribution of the signal. Three categories were defined: cells showing a nuclear staining with low cytoplasmic signal (N>C); cells showing an equal distribution between the nuclear and cytosolic compartment (N=C); cells having exclusive cytoplasmic signal (N<C). These results demonstrate that co-expression of Myc-NES-Obi1(1-280) causes Obi1 to exhibit a stronger cytoplasmic staining, indicating that Myc-NES-Obi1(1-280) acts as a dominant negative form and sequestrate WT-Obi1 protein in the cytoplasm.
Finally, the inventors evaluated the physiological effect of the Myc-NES-Obi1(1-280) expression. U20S cells were transiently transfected with plasmids coding for EGFP along with Myc-tagged NES-Obi1(1-280) or the empty vector, as indicated. 72 hours post-transfection, cells were trypsined and analyzed for fluorescence by flow cytometry (
These data show that expression of NES-Obi1(1-280) induces a selective loss of transfected cells, possibly by inducing cell cycle arrest or cell death.
These data also strongly suggest that a dominant negative form of Obi1 may influence cell proliferation, and in particular cell proliferation of cancer cells.
To further evaluate the importance of Obi1 gene in regulation of DNA replication, the inventors have evaluated the possible involvement of Obi1 mutation in Meier-Gorlin syndrome patients.
Within a cohort of family having at least one member afflicted by Meier-Gorlin syndrome, the inventors have identified a patient who was heterozygous for a frameshift which lies in the last exon and would predict a truncated protein lacking the last 270 (SEQ ID NO: 100).
The mutation identified by the inventors is C.1370_1371delAA,P.GLU457VALFSX24, i.e. a deletion of the consecutive A at position 1370 and 1371 of the nucleic acid molecule as set forth in SEQ ID NO: 97, resulting in the nucleic acid molecule as set forth in SEQ ID NO: 99. The mutated mRNA expressed in the patient is the nucleic acid molecule as set forth in SEQ ID NO: 98.
The remainder of the gene is covered nicely and there doesn't appear to any second hits. The mother is a carrier for the identified mutation and there is nothing of note in the father.
What is interesting is that in the patient is a query of autosomal dominant inheritance in this family, with the mother being non-penetrant, as apparently the maternal grandmother and the maternal great-grandfather look strikingly similar.
The patient's growth parameters are more mild, like Meier-Gorlin Syndrome, −3.1 Osteitis fibrosa cystica −4.4 height but with osteopenia and a few other bone abnormalities. There is nothing of note in regards to hypomorphic ears or patella.
In order to characterize the protein expressed by the mutated allele identified in the Meier-Gorlin patient, the inventors have tested its ability to interact with the ORC complex.
U20S cells were transiently transfected with plasmids coding for Myc-tagged WT Obi1 or mutated Obi1, and also co-transfected with with plasmids coding for Flag-ORC1. 48 hours post-transfection, cells were lyzed and the soluble fraction was subjected to an anti-Flag immunoprecipitation (IP:Flag—
These results demonstrate that truncated Obi1 protein does not interact with ORC, which leads to a modification in DNA replication metabolism.
The natural mutant observed in Meier-Gorlin syndrome appears to act in a similar way than the artificial dominant negative mutant NES-Obi1(1-280) described above, by interfering with the endogenous Obi1 protein activity.
Number | Date | Country | Kind |
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13305725.7 | May 2013 | EP | regional |
Filing Document | Filing Date | Country | Kind |
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PCT/EP2014/061369 | 6/2/2014 | WO | 00 |