SOLID-PHASE SYNTHESIS CARRIER, PREPARATION METHOD THEREFOR AND USE THEREOF

Abstract
A solid-phase synthesis carrier, a preparation method therefor and the use thereof, wherein a diene cross-linking agent with a similar reactivity ratio to styrene and two vinyl groups thereof not on the same benzene ring is selected as a cross-linking monomer, and is subjected to suspension polymerization to obtain a porous resin. The porous resin is then functionalized to obtain a porous resin with an amino or hydroxyl functional group. Compared with existing preparation methods, the reactivity ratio of the cross-linking agent and styrene is similar, which is beneficial to improving the uniformity of the chemical structure in the resin, forming uniformly distributed active sites and channels, and is beneficial to improving the reaction efficiency and reducing the mass transfer resistance. The preparation of oligonucleotides by using such a carrier as a solid-phase synthesis carrier can improve the yield and purity of the oligonucleotides.
Description
TECHNICAL FIELD

The invention relates to a solid-phase synthesis carrier, preparation method thereof and use thereof. The carrier is for use in the solid-phase synthesis of oligonucleotides and belongs to the field of preparation of functional polymer materials


BACKGROUND

As one of the effective tools for precision medicine, more and more oligonucleotide drugs are being approved for marketing. Oligonucleotides drugs are often synthesized using chemical methods, and the most common method is solid-phase phosphoramidite synthesis, in which a solid-phase synthesis carrier is filled in a reaction column and a solution with dissolved reactants is rapidly flowed through the column under a certain pressure to complete the reaction.


At the early stage of the development of oligonucleotide solid-phase synthesis technology, the commonly used solid-phase synthesis carriers include inorganic particles such as controlled pore glass microspheres (CPG) and modified silica, but they have obvious drawbacks such as low loading (generally less than 100 μmmol/g), which leads to the limited yield of single batch of oligonucleotide, low equipment utilization and high production cost. In order to improve the loading of the carrier, Nitto Denko CO. LTD. and Ionis Inc. jointly filed a patent application WO2006029023, which involved preparing organic polymers as carries for oligonucleotides solid-phase synthesis, using styrene, acetoxystyrene and divinylbenzene as polymerization monomers and isooctane and 2-ethyl-1-hexanol as pore-forming agents. The prepared carrier had a loading of up to 100-350 μmmol/g. In order to further improve the yield and purity of oligonucleotides, patent application U.S. Pat. No. 8,653,152 filed by Nitto Denko CO. LTD use styrene, methacrylonitrile, acetoxystyrene and divinylbenzene as polymerization monomers, isooctane, 2-ethyl-1-hexanol as pore-forming agent to prepare a solid-phase synthesis carrier. The synthesis efficiency is improved by adding methacrylonitrile to suppress the swelling fluctuation of the solid-phase synthesis carrier in different solvents.


Both of the above polymer carriers use divinylbenzene as a cross-linking agent. During use, divinylbenzene has two main problems, one is that the purity is not high, and the other is that it has three isomers with different properties. This leads to a great difference in the performance of the resins produced using different quality divinylbenzene from different manufacturers. At present, the purity of general industrial divinylbenzene is 40-60%. In addition to divinylbenzene, it also contains a certain amount of ethyl styrene, and some also contain a small amount of diethylbenzene.


The three isomers of divinylbenzene show different reactivity when copolymerizing with other monomers, which has a significant impact on the structure and performance of the copolymer. In a study on the copolymerization kinetics of styrene-divinylbenzene by He Binglin et al. (Reactive Polymer, 12 (1990), 269-275), it was found that p-divinylbenzene and m-divinylbenzene have faster conversion rate than styrene in the copolymerization process. This leads to high cross-linking degree of copolymers formed in the early stage of polymerization and low cross-linking degree of copolymers formed in the late stage of polymerization, thus leading to heterogeneous chemical structure in the resin. Due to the heterogeneous chemical structure, the macroporous adsorption resin with styrene-divinylbenzene as the skeleton has a series of problems during use, such as varying degrees of fragmentation, long time to reach the adsorption equilibrium, tailing after desorption, incomplete regeneration, etc.


Diene cross-linking agents such as 1, 2-bis (4-vinylphenyl) ethane, where two vinyl groups are not on the same benzene ring, have a reactivity similar to styrene. Sundell et al. (Journal of Polymer Science Part A: Polymer Chemistry, 31 (1993), 2305-2311) prepared strong acid resins using this kind of monomers as cross-linking agents. Experimental results showed that these resins had higher mechanical strength than strong acid resins based on styrene-divinylbenzene copolymers. In a Research on Synthesis and Adsorption Performance of 1,2-bis (p-vinylphenyl) ethane Polymers, ultrahigh crosslinked polystyrene adsorption resins were prepared with 1,2-bis (p-vinylphenyl) ethane and divinylbenzene as cross-linking agents respectively. Experimental results showed that the adsorption resins with 1,2-bis (p-vinylphenyl) ethane as a cross-linking agent had no tailing phenomenon during use and were easy to regenerate.


Oligonucleotide drugs have emerged in the treatment of diseases such as anti-virus, high cholesterol, gene expression editing, visual blindness and hepatic vein obstruction due to their high therapeutic efficiency, low drug toxicity, strong specificity and wide application fields. The demand for oligonucleotide drugs is increasing year by year. At the same time, the existing carriers for oligonucleotide solid-phase synthesis have problems such as heterogeneous internal structure and high mass transfer resistance, which lead to low oligonucleotide synthesis efficiency and high production cost. Therefore, it is necessary to develop a solid-phase synthesis carrier which allows large scale synthesis of oligonucleotide drugs at low cost and with high efficiency to meet the market demand of oligonucleotide drugs.





BRIEF DESCRIPTION OF THE DRAWINGS

The present disclosure is best understood from the following detailed description when read with the accompanying Figures. It is emphasized that, in accordance with the standard practice in the industry, various features are not drawn to scale. In fact, the dimensions of the various features may be arbitrarily increased or reduced for clarity of discussion.



FIG. 1 shows a scanning electron microscope image of the carrier in Example 1,



FIG. 2 shows a scanning electron microscope image of the carrier in Example 2,



FIG. 3 shows a scanning electron microscope image of the carrier in Example 3,



FIG. 4 shows a scanning electron microscope image of the carrier in Example 4,



FIG. 5 shows a scanning electron microscope image of the carrier in Example 5,



FIG. 6 shows a scanning electron microscope image of the carrier in Example 6,



FIG. 7 shows a scanning electron microscope image of the carrier in Example 7,



FIG. 8 shows a scanning electron microscope image of the carrier in Example 8,



FIG. 9 shows a scanning electron microscope image of the carrier in Example 9,



FIG. 10 shows the pore size distribution of the carrier in Example 1 measured by mercury intrusion method;



FIG. 11 shows the pore size distribution of the carrier in Example 2 measured by mercury intrusion method;



FIG. 12 shows the pore size distribution of the carrier in Example 3 measured by mercury intrusion method;



FIG. 13 shows the pore size distribution of the carrier in Example 4 measured by mercury intrusion method;



FIG. 14 shows the pore size distribution of the carrier in Example 5 measured by mercury intrusion method;



FIG. 15 shows the pore size distribution of the carrier in Example 6 measured by mercury intrusion method;



FIG. 16 shows the pore size distribution of the carrier in Example 7 measured by mercury intrusion method;



FIG. 17 shows the pore size distribution of the carrier in Example 8 measured by mercury intrusion method;



FIG. 18 shows the pore size distribution of the carrier in Example 9 measured by mercury intrusion method.





DETAILED DESCRIPTION

In order to achieve the large-scale production of oligonucleotides at low-cost and overcome the disadvantages such as heterogeneous internal structure and high mass transfer resistance of existing carriers for solid-phase synthesis of oligonucleotides, the present invention provides a solid-phase synthesis carrier and preparation method thereof and use thereof.


The present invention selects diene compounds, which have two vinyl groups that are not on the same benzene ring, as cross-linking monomers, showing mainly the following three effects: Firstly, such type of monomers have a reactivity ratio similar to styrene, which is conducive to improving the uniformity of the chemical structure inside the resin and forming uniformly distributed active sites. Secondly, the improvement in homogeneity of the chemical structure inside the resin is beneficial to formation of uniform pore channels inside the resin, which reduces the mass transfer resistance. Thirdly, compared with divinylbenzene, such type of cross-linking agents contain flexible molecular chains which can improve the swelling performance of the resin in different organic solvents.


The present invention provides a solid-phase synthesis carrier, wherein the carrier has a polymer skeleton with functional groups which is represented by the following formula:

    • wherein, R1=-(CH2)n-, n is an integer of 0-3, or R1=-O—(CH2)m-O—, m is an integer of 1-4; and R2=-OH or —NH2.


In some embodiments, the solid-phase synthesis carrier is a copolymer comprising repeating structural units represented by formula (I), formula (II), formula (III), and formula (IV) in its skeleton:




embedded image




    • wherein, R3 is selected from the groups consisting of —H, —CN and —CH2-CN; R4 is —H or —CH3; and R5 is selected from the groups consisting of —CN, —CH2-CN, —OOCH3 and —CONH2;







embedded image




    • wherein, R6 is —(CH2)x-, x is an integer 0-3, or R6 is —O—(CH2)y-O—, y is an integer 1-4;







embedded image




    • R7 is selected from the groups consisting of —H, CH3(CH2)z- or CH3(CH2)ZO—, wherein z is an integer 0-4, (CH3)2CH—, (CH3)2CH(CH2)-, (CH3)2CH(CH2)2-, (CH3)3C—, CH3CH2CH(CH3)-, CH3CH2C(CH3)2-, and CH3CH2CH2CH(CH3)-;







embedded image




    • R8 is selected from the groups consisting of —OH, —CH2OH, —NH2, —CH2NH2, —CHCOOC—C6H4-OH, —CHCOOCCH2-C6H4-OH, —(CH2)4OOC—C6H4-OH, —(CH2)4OOCCH2-C6H4-OH, —(CH2)4OOCCH2-C6H4-NH2, —CH2COONH—C6H4-NH2, —COO—C6H4-OH and —CH2COO—C6H4-OH.





In some embodiments, the carrier has a content of hydroxyl group or amino group of 100-1000 μmmol/g, preferably 400-700 μmmol/g.


In some embodiments, the carrier has a particle size in a range of 35-200 μm, preferably 50-100 μm.


In some embodiments, the carrier has an average pore diameter of 10-200 nm, preferably 40-100 nm.


The present invention also provides a preparation method of the solid-phase synthesis. The preparation method comprises following steps of: preparing an aqueous phase and an oil phase, respectively; the aqueous phase comprising water, a dispersant and an inorganic salt; the oil phase comprising: a cross-linking monomer, a monovinyl compound, a functional monomer, a modified monomer, a pore-forming agent and an initiator, wherein the cross-linking monomer, the monovinyl compound, the functional monomer and the modified monomer are monomers capable of polymerization; and adding the oil phase to the aqueous phase, stirring and heating to carry out reaction, and removing the pore-forming agent after the reaction is completed, obtaining a porous polymer resin. The porous polymer resin is capable of undergoing a further reaction to obtain a solid-phase synthesis carrier containing a hydroxyl group or an amino group as functional groups.


In some embodiments, more specifically, the cross-linking monomer is a diene cross-linking agent which has two vinyl groups not on the same benzene ring, selected from the group consisting of 4,4′-divinylbiphenyl, di(4-vinylphenyl) methane, 1,2-di(4-vinylphenyl) ethane, 1,3-di(4-vinylphenyl) propane, di(4′-vinylphenoxy) methane, 1,2-di(4′-vinylphenoxy) ethane, 1,3-di(4′-vinylphenoxy) propane, 1,4-di(4′-vinylphenoxy) butane and any combination thereof. Preferably, the cross-linking monomer is 1,2-di(4-vinylphenyl) ethane.


In some embodiments, the monovinyl compound is an aromatic monovinyl compound. The monovinyl compound is styrene, unsubstituted or substituted with C1-C5 alkyl on its benzene ring, such as methyl styrene, ethyl styrene, n-propyl styrene, isopropyl styrene, n-butyl styrene, isobutyl styrene, sec butyl styrene, tert butyl styrene, n-amyl styrene, isopentyl styrene, sec amyl styrene or tert amyl styrene; or styrene substituted with C1-C5 alkoxy, such as methoxy styrene, ethoxy styrene, propoxy styrene, butoxy styrene or pentoxy styrene. Preferably, the monovinyl compound is styrene.


In some embodiments, the functional monomer has a double bond capable of free radical polymerization, and also has a hydroxyl group, an amino group, a halogenated group or other group capable of converting into a hydroxyl group and an amino group via reaction. In the process of oligonucleotide synthesis, the reactive hydroxyl group or amino group works as active sites to connect oligonucleotides, including amino group, aminoalkyl group, hydroxyl group and hydroxyalkyl group etc. Primary amino group, aminomethyl group, hydroxyl group and hydroxymethyl group, etc. are preferred. The functional monomer comprises but is not limited to hydroxystyrene and derivatives thereof, such as 4-hydroxystyrene etc.; hydroxyalkyl styrene and derivatives thereof, such as 4-hydroxymethyl styrene etc.; acyloxy styrene and derivatives thereof, such as 4-acetoxy styrene and benzoyloxy styrene etc.; amino styrene and derivatives thereof, such as 4-amino styrene etc.; aminoalkyl styrene and derivatives thereof, such as 4-aminomethyl styrene etc.; haloalkyl styrene monomers, such as 4-(4-bromobutyl) styrene and 4-chloromethyl styrene etc.; 4-vinylphenyl ester monomers, such as methyl 4-vinylbenzoate and 4-ethenylbenzeneacetic acid ethyl ester etc.


In some embodiments, some of the functional monomers contain hydroxyl protection groups or amino protection groups which can be directly cut off to form amino groups or hydroxyl groups. For example, acyloxy styrene can be converted via alkali hydrolysis or acid hydrolysis into hydroxyl groups for serving as the active sites for connecting oligonucleotides; Some of the functional monomers need to be converted through a functionalization reaction into amino groups or hydroxyl groups for serving as active sites. For example, haloalkyl styrene can be converted through hydrolysis into hydroxyl group or converted through Gabriel reaction into primary amino groups for serving as active sites for connecting oligonucleotides; Some of the functional monomers need to link connecting arms having amino or hydroxyl groups for serving as active sites. For example, haloalkyl styrene can react with 4-hydroxybenzoic acid or 4-hydroxyphenylacetic acid to generate hydroxyl groups for serving as active sites for connecting oligonucleotides; Some of the functional monomers need the above multiple reactions to obtain amino groups or hydroxyl groups for serving as active sites. For example, 4-vinylphenyl esters monomers need to hydrolyze to expose carboxyl groups first, and then react with hydroquinone or p-phenylenediamine to obtain amino groups or hydroxyl groups for serving as active sites.


In some embodiments, the modified monomer has a double bond capable of free radical polymerization and also has cyano group, ester group and amide group. The modified monomer comprises but is not limited to acrylonitrile, methacrylonitrile, fumaronitrile, 1,4-dicyano-2-butene, methyl methacrylate and acrylamide.


In some embodiments, the initiator is selected from the group consisting of organic peroxides and azo compounds. The initiator comprises but is not limited to benzoyl peroxide, lauroyl peroxide, tert butyl peroxy-2-ethylhexanoate, 2,2′-azobis(2-methylpropionitrile), 2,2′-azobis(2-methylbutyronitrile) and 2,2′-azobis(2,4-dimethyl)valeronitrile. The initiator accounts for 0.5-5% by weight based on a total weight of the monomers.


In some embodiments, the pore-forming agent is an organic solvent or a surfactant which is not polymerizable and insoluble or slightly soluble in water. The pore-forming agent is selected from the group consisting of aromatic hydrocarbon such as benzene, toluene and ethylbenzene; aliphatic hydrocarbons, such as C6-C12 linear or branched alkanes or C6-C12 cycloalkanes, such as hexane, heptane, octane, dodecane, isooctane, isododecane and cyclohexane; halogenated hydrocarbons such as chloroform and chlorobenzene; esters containing 4 or more carbon atoms, such as ethyl acetate, butyl acetate and dibutyl phthalate; alcohols, such as C4-C12 linear or branched alkane alcohol or C4-C12 cycloalkane alcohol, such as hexanol, cyclohexanol, octanol, isooctanol, decanol and dodecanol; oil-soluble surfactants such as sorbitan trioleate, polyoxyethylene sorbitol beeswax derivative, sorbitan tristearate, polyoxyethylene sorbitol hexastearate, ethylene glycol fatty acid ester, propylene glycol fatty acid ester, propylene glycol monostearate, sorbitan sesquioleate, polyoxyethylene sorbitol oleate, monostearin, lanolin hydroxylated, sorbitol monooleate and propylene glycol laurate, and any combination thereof.


In some embodiments, the aqueous phase comprises water, a dispersant and an inorganic salt. The dispersant is a water-soluble polymer which comprises but is not limited to one or more selected from the group consisting of polyvinyl alcohol, hydroxyethyl cellulose, hydroxyethyl methyl cellulose, carboxymethyl cellulose, methyl cellulose, ethyl cellulose, sodium polyacrylate and polyvinylpyrrolidone. The dispersant is present in the aqueous phase in an amount of 0.1-5% by weight. The inorganic salt acts to regulate the density of the aqueous phase while reducing the solubility of the components of the oil phase in the aqueous phase, so that oil droplets are more stably dispersed in the aqueous phase. The inorganic salt comprises but is not limited to one or more selected from the group consisting of sodium chloride, potassium chloride, calcium chloride, sodium sulfate, potassium sulfate and calcium sulfate, etc. The inorganic salt is present in the aqueous phase in an amount of 20% by weight or lower.


In some embodiments, in order to reduce the bonding between resins and improve the heat transfer of polymerization, as well as to improve equipment utilization and production efficiency, a weight ratio of the oil phase to the aqueous phase is set to 1:3-1:20.


In some embodiments of the present invention, the different components are present in the following amounts: the monovinyl compound originally comprised in the oil phase accounts for 45-95% by weight based on a total weight of the monomers; the cross-linking monomer originally comprised in the oil phase accounts for 2.9-20% by weight based on a total weight of the monomers; the functional monomers originally comprised in the oil phase accounts for 2-20% by weight based on a total weight of the monomers; the modified monomer originally comprised in the oil phase accounts for 0.1-15% by weight based on a total weight of the monomers; and the pore-forming agent originally comprised in the oil phase accounts for 15-130% by weight based on a total weight of the monomers.


In some more preferred embodiments of the present invention, the different components are present in the following amounts: the monovinyl compound originally comprised in the oil phase accounts for 62-86% by weight based on a total weight of the monomers; the cross-linking monomer originally comprised in the oil phase accounts for 7-13% by weight based on a total weight of the monomers; the functional monomers originally comprised in the oil phase accounts for 5-15% by weight based on a total weight of the monomers; the modified monomer originally comprised in the oil phase accounts for 2-10% by weight based on a total weight of the monomers; and the pore-forming agent originally comprised in the oil phase accounts for 30-110% by weight based on a total weight of the monomers.


In some embodiments, the polymerization is carried out at a temperature of 50-90° C., preferably, 70-85° C.


In some embodiments, the preparation method of the solid-phase synthesis carrier comprises following steps of:

    • adding a certain amount of purified water into a reactor, adding the dispersant in an amount which is 0.1-5% by weight of the aqueous phase and the inorganic salt in an amount which is not more than 20% by weight of the aqueous phase, and dissolving to obtain an aqueous phase;
    • weighing out the monovinyl compound, cross-linking monomer, functional monomer, modified monomer, pore-forming agent and initiator according to a weight ratio of the oil phase to the aqueous phase being 1:3-1:20; wherein, the monovinyl compound accounts for 45-95% of the total weight of the monomers, the cross-linking monomer accounts for 2.9-20% of the total weight of the monomers, the functional monomer accounts for 2-20% of the total weight of the monomers, and the modified monomer accounts for 0.1-15% of the total weight of the monomers, the pore-forming agent accounts for 15-130% of the total weight of monomers, and mixing well to obtain an oil phase;
    • adding the oil phase into the reactor, stirring and heating up to 50-90° C. to carry out reaction; removing the pore-forming agent after the reaction is completed, and screening and collecting the resin with appropriate particle size, and vacuum drying to obtain a porous polymer resin; and
    • carrying out a further reaction with the resin to obtain a solid-phase synthesis carrier having amino group or carboxyl group.


In some embodiments, the preparation method of the solid-phase synthesis carrier comprises following steps of:

    • adding a certain amount of purified water into a reactor, adding the dispersant in an amount which is 0.1-5% by weight of the aqueous phase and the inorganic salt in an amount which is not more than 20% by weight of the aqueous phase, and dissolving to obtain an aqueous phase;
    • weighing out the monovinyl compound, cross-linking monomer, functional monomer, modified monomer, pore-forming agent and initiator according to a weight ratio of the oil phase to the aqueous phase being 1:3-1:20; wherein, the monovinyl compound accounts for 62-86% of the total weight of the monomers, the cross-linking monomer accounts for 7-13% of the total weight of the monomers, the functional monomer accounts for 5-15% of the total weight of the monomers, and the modified monomer accounts for 2-10% of the total weight of the monomers, the pore-forming agent accounts for 30-110% of the total weight of monomers, and mixing well to obtain an oil phase;
    • adding the oil phase into the reactor, stirring and heating up to 70-85° C. to carry out reaction; removing the pore-forming agent after the reaction is completed, and screening and collecting the resin with appropriate particle size, and vacuum drying to obtain a porous polymer resin; and
    • carrying out a further reaction with the resin to obtain a solid-phase synthesis carrier having amino group or carboxyl group.


The above method enables to obtain the solid-phase synthesis of the present invention, i.e., a porous resin having hydroxyl groups or amino groups. In the present invention, the content of amino group or hydroxyl group, i.e., the loading, can be calculated by reacting with Fmoc-Leu-OH and then removing the Fmoc protecting group. The amount of Fmoc removed is determined by colorimetric method, and then the content of amino group or hydroxyl group in the carrier is calculated.


In some embodiments, the detailed operation is as follows: 1.0 g of the carrier is accurately weighed and suspended in 7 ml of acetonitrile solution, then 0.5 g of Fmoc-Leu-OH, 0.5 g of HBTU and 0.5 ml of DIEA are added thereto, and stirred at room temperature to carry out reaction for 2 h. After the reaction is completed, the resin is washed successively with acetonitrile (10 ml for each time, three times) and methanol (10 ml for each time, three times), and then the resin is dried. 0.1000 g of the resin is weighed accurately, suspended in 20% piperidine/DMF (v/v) solution, and shaken for at room temperature, filtered, and the filtrate is collected. The resin is washed with DMF and the filtrate is collected. The filtrates are combined to provide a total volume, and then diluted appropriate times to measure the absorbance at 300 nm. Similar Fmoc removal reactions are carried out by using a series of known concentrations of Fmoc-Leu-OH and the absorbance are measured to make a standard curve. The content of amino group or hydroxyl group in the carrier is calculated via the standard curve.


The functional group content of the carrier depends on the percentages of the functional monomers based on a total weight of the monomers, and a series of carriers with different amino group or hydroxyl group contents can be obtained by adjusting the amount of functional monomers. The functional group content of the carrier determines the amount of synthesized oligonucleotides; If the functional group content is too low, the yield of oligonucleotides in a single batch will be reduced; and if the functional group content is too high, the purity of oligonucleotides will be affected. In the present invention, the functional group content of the carrier ranges from 100-1000 μmmol/g, preferably 400-700 μmmol/g.


The particle size of the carrier in present invention is measured by particle image processing instrument. The carrier is uniformly distributed on a slide, and observed under a microscope at magnification, while images of the carrier particles under magnification are captured by a camera. Morphological features and particle size of the carrier are analyzed and calculated by a computer.


The particle size of the carrier mainly depends on the type and amount of dispersant present in the aqueous phase, the type and amount of pore-forming agents and the speed of stirring during the suspension polymerization. The particle size of the carrier can be regulated by adjusting above conditions. If the particle size of the carrier is too large, on the one hand, it will lead to the decrease of the specific surface area of the carrier and the increase of the number of active sites per unit area, which will affect the purity of oligonucleotide; on the other hand, if the particle size is too large, it will slow down the mass transfer rate and lead to the increase of impurities during the synthesis of oligonucleotides. If the particle size of the carrier is too small, it will cause too high pressure in the synthesis process and greatly increase the cost of equipment. In the present invention, the carrier has a particle size in a range of 35-200 μm, preferably 50-100 μm.


The average pore diameter of the carrier is measured by mercury intrusion method. 0.1500-0.3000 g samples are precisely weighed and put into an automatic mercury porosimeter AutoPore IV 9500 (Micromeritics Instrument Co.). The contact angle of mercury is set to 130° and surface tension is set to 485 dyn/cm, and then measured by mercury intrusion method under these conditions. The average pore diameter of the carrier mainly depends on the type and amount of pore-forming agents, the amount of cross-linking agent, the reaction temperature and time, etc. The average pore diameter of the carrier can be regulated by adjusting these conditions. If the average pore diameter of the carrier is too small, it will cause difficulties in mass transfer and affect the synthesis efficiency; if the average pore diameter of the carrier is too large, it will lead to the decrease of the specific surface area of the carrier and the increase of the active sites per unit area. During oligonucleotide synthesis, nucleoside growth will cause mutual influence and affect oligonucleotide purity. In the present invention, the carrier has an average pore diameter of 10-200 nm, preferably 40-100 μm.


Compared with prior art, the present invention has three main advantages: Firstly, the present invention selects monomers which have a reactivity ratio similar to styrene as cross-linking agents, which is conducive to improving the uniformity of the internal chemical structure of the resin and forming uniformly distributed active sites. Secondly, the improvement in homogeneity of the internal chemical structure of the resin is conducive to the formation of uniform pore channels in the resin, thereby reducing the mass transfer resistance. Thirdly, compared with divinylbenzene, this kind of cross-linking agents contain flexible chains in its structure, which can improve the swelling performance of the resin in different organic solvents.


Examples in the present disclosure may also be directed to a non-transitory computer-readable medium storing computer-executable instructions and executable by one or more processors of the computer via which the computer-readable medium is accessed. A computer-readable media may be any available media that may be accessed by a computer. By way of example, such computer-readable media may comprise RAM, ROM, EEPROM, CD-ROM or other optical disk storage, magnetic disk storage or other magnetic storage devices, or any other medium that may be used to carry or store desired program code in the form of instructions or data structures and that may be accessed by a computer. Disk and disc, as used herein, includes compact disc (CD), laser disc, optical disc, digital versatile disc (DVD), floppy disk and Blu-ray® disc where disks usually reproduce data magnetically, while discs reproduce data optically with lasers.


Note also that the software implemented aspects of the subject matter claimed below are usually encoded on some form of program storage medium or implemented over some type of transmission medium. The program storage medium is a non-transitory medium and may be magnetic (e.g., a floppy disk or a hard drive) or optical (e.g., a compact disk read only memory, or “CD ROM”), and may be read only or random access. Similarly, the transmission medium may be twisted wire pairs, coaxial cable, optical fiber, or some other suitable transmission medium known to the art. The claimed subject matter is not limited by these aspects of any given implementation.


The foregoing description, for purposes of explanation, used specific nomenclature to provide a thorough understanding of the disclosure. However, it will be apparent to one skilled in the art that the specific details are not required in order to practice the systems and methods described herein. The foregoing descriptions of specific examples are presented for purposes of illustration and description. They are not intended to be exhaustive of or to limit this disclosure to the precise forms described. Obviously, many modifications and variations are possible in view of the above teachings. The examples are shown and described in order to best explain the principles of this disclosure and practical applications, to thereby enable others skilled in the art to best utilize this disclosure and various examples with various modifications as are suited to the particular use contemplated. It is intended that the scope of this disclosure be defined by the claims and their equivalents below.

Claims
  • 1. A solid-phase synthesis carrier, wherein the carrier has a polymer skeleton with functional groups which is represented by the following formula:
  • 2. The solid-phase synthesis carrier according to claim 1, wherein the carrier has a content of hydroxyl group or amino group of 100-1000 μmmol/g, preferably, 400-700 μmmol/g.
  • 3. (canceled)
  • 4. The solid-phase synthesis carrier according to claim 1, wherein the carrier has a particle size in a range of 35-200 μm, preferably 50-100 μm.
  • 5. (canceled)
  • 6. The solid-phase synthesis carrier according to claim 1, wherein the carrier has an average pore diameter of 10-200 nm, preferably 40-100 nm.
  • 7. (canceled)
  • 8. A method for preparing the solid-phase synthesis carrier according to claim 1, comprising the following steps of: A. preparing an aqueous phase and an oil phase, respectively; the aqueous phase comprising water, a dispersant and an inorganic salt; the oil phase comprising: a cross-linking monomer, a monovinyl compound, a functional monomer, a modified monomer, a pore-forming agent and an initiator, wherein the cross-linking monomer, the monovinyl compound, the functional monomer and the modified monomer are monomers capable of polymerization; andB. adding the oil phase to the aqueous phase, stirring and heating to carry out reaction, and removing the pore-forming agent after the reaction is completed, obtaining a porous polymer resin.
  • 9. The method according to claim 8, wherein the porous polymer resin is capable of undergoing a further reaction to obtain a solid-phase synthesis carrier containing a hydroxyl group or an amino group as functional groups.
  • 10. The method according to claim 8, wherein the cross-linking monomer is a diene cross-linking agent which has two vinyl groups not on the same benzene ring, and preferably, the cross-linking monomer is selected from the group consisting of 4,4′-divinylbiphenyl, di(4-vinylphenyl) methane, 1,2-di(4-vinylphenyl) ethane, 1,3-di(4-vinylphenyl) propane, di(4′-vinylphenoxy) methane, 1,2-di(4′-vinylphenoxy) ethane, 1,3-di(4′-vinylphenoxy) propane, 1,4-di(4′-vinylphenoxy) butane and any combination thereof.
  • 11. (canceled)
  • 12. The method according to claim 8, wherein the monovinyl compound is an aromatic monovinyl compound, and preferably, the monovinyl compound is styrene, unsubstituted or substituted with C1-C5 alkyl or alkoxy on its benzene ring.
  • 13. (canceled)
  • 14. The method according to claim 8, wherein the functional monomer has a double bond capable of free radical polymerization, and also has a hydroxyl group, an amino group, a halogenated group or other group capable of converting into a hydroxyl group and an amino group via reaction, and preferably, the functional monomer is selected from the group consisting of hydroxystyrene and derivatives thereof, such as 4-hydroxystyrene; hydroxyalkyl styrene and derivatives thereof, such as 4-hydroxymethyl styrene; acyloxy styrene and derivatives thereof, such as 4-acetoxy styrene and benzoyloxy styrene; amino styrene and derivatives thereof, such as 4-amino styrene; aminoalkyl styrene and derivatives thereof, such as 4-aminomethyl styrene; haloalkyl styrene monomers, such as 4-(4-bromobutyl) styrene and p-chloromethyl styrene; 4-vinylphenyl ester monomers, such as methyl 4-vinylbenzoate, and 4-ethenylbenzeneacetic acid ethyl ester.
  • 15. (canceled)
  • 16. The method according to claim 8, wherein the modified monomer has a double bond capable of free radical polymerization and also has cyano group, ester group and amide group, and preferably, the modified monomer is selected from the group consisting of acrylonitrile, methacrylonitrile, fumaronitrile, 1,4-dicyano-2-butene, methyl methacrylate and acrylamide.
  • 17. (canceled)
  • 18. The method according to claim 8, wherein the initiator is an organic peroxide or an azo compound, and preferably, the initiator is selected from the group consisting of benzoyl peroxide, lauroyl peroxide, tert butyl peroxy-2-ethylhexanoate, 2,2′-azobis(2-methylpropionitrile), 2,2′-azobis(2-methylbutyronitrile) and 2,2′-azobis(2,4-dimethyl)valeronitrile.
  • 19. (canceled)
  • 20. The method according to claim 8, wherein the pore-forming agent is an organic solvent or a surfactant which is not polymerizable and insoluble or slightly soluble in water, and preferably, the pore-forming agent is selected from the group consisting of aromatic hydrocarbon such as benzene, toluene and ethylbenzene; aliphatic hydrocarbons, such as C6-C12 linear or branched alkanes or C6-C12 cycloalkanes, such as hexane, heptane, octane, dodecane, isooctane, isododecane and cyclohexane; halogenated hydrocarbons such as chloroform and chlorobenzene; esters containing 4 or more carbon atoms, such as ethyl acetate, butyl acetate and dibutyl phthalate; alcohols, such as C4-C12 linear or branched alkane alcohol or C4-C12 cycloalkane alcohol, such as hexanol, cyclohexanol, octanol, isooctanol, decanol and dodecanol; oil-soluble surfactants such as sorbitan trioleate, polyoxyethylene sorbitol beeswax derivative, sorbitan tristearate, polyoxyethylene sorbitol hexastearate, ethylene glycol fatty acid ester, propylene glycol fatty acid ester, propylene glycol monostearate, sorbitan sesquioleate, polyoxyethylene sorbitol oleate, monostearin, lanolin hydroxylated, sorbitol monooleate and propylene glycol laurate, and any combination thereof.
  • 21. (canceled)
  • 22. The method according to claim 8, wherein, the dispersant is present in an amount of 0.1-5% by weight in the aqueous phase, and the inorganic salt is present in an amount of 20% by weight or lower in the aqueous phase;a weight ratio of the oil phase to the aqueous phase is 1:3-1:20;the monovinyl compound in the oil phase accounts for 45-95%, preferably 62-86% by weight based on a total weight of the monomers;the cross-linking monomer in the oil phase accounts for 2.9-20%, preferably 7-13% by weight based on a total weight of the monomers;the functional monomers in the oil phase accounts for 2-20%, preferably 5-15% by weight based on a total weight of the monomers;the modified monomer in the oil phase accounts for 0.1-15%, preferably 2-10% by weight based on a total weight of the monomers; andthe pore-forming agent in the oil phase accounts for 15-130%, preferably 30-110% by weight based on a total weight of the monomers.
  • 23. (canceled)
  • 24. The method according to claim 8, wherein the polymerization is carried out at a temperature of 50-90° C., preferably 70-85° C.
  • 25. (canceled)
  • 26. The method according to claim 8, comprising the following steps of: adding a certain amount of purified water into a reactor, adding the dispersant in an amount which is 0.1-5% by weight of the aqueous phase and the inorganic salt in an amount which is not more than 20% by weight of the aqueous phase, and dissolving to obtain an aqueous phase;weighing out the monovinyl compound, cross-linking monomer, functional monomer, modified monomer, pore-forming agent and initiator according to a weight ratio of the oil phase to the aqueous phase being 1:3-1:20; wherein, the monovinyl compound accounts for 45-95% of the total weight of the monomers, the cross-linking monomer accounts for 2.9-20% of the total weight of the monomers, the functional monomer accounts for 2-20% of the total weight of the monomers, and the modified monomer accounts for 0.1-15% of the total weight of the monomers, the pore-forming agent accounts for 15-130% of the total weight of monomers, and mixing well to obtain an oil phase;adding the oil phase into the reactor, stirring and heating up to 50-90° C. to carry out reaction; removing the pore-forming agent after the reaction is completed, and screening and collecting the resin with appropriate particle size, and vacuum drying to obtain a porous polymer resin; andcarrying out a further reaction with the resin to obtain a solid-phase synthesis carrier having amino group or carboxyl group.
  • 27. The method according to claim 26, comprising the following steps of: adding a certain amount of purified water into a reactor, adding the dispersant in an amount which is 0.1-5% by weight of the aqueous phase and the inorganic salt in an amount which is not more than 20% by weight of the aqueous phase, and dissolving to obtain an aqueous phase;weighing out the monovinyl compound, cross-linking monomer, functional monomer, modified monomer, pore-forming agent and initiator according to a weight ratio of the oil phase to the aqueous phase being 1:3-1:20; wherein, the monovinyl compound accounts for 62-86% of the total weight of the monomers, the cross-linking monomer accounts for 7-13% of the total weight of the monomers, the functional monomer accounts for 5-15% of the total weight of the monomers, and the modified monomer accounts for 2-10% of the total weight of the monomers, the pore-forming agent accounts for 30-110% of the total weight of monomers, and mixing well to obtain an oil phase;adding the oil phase into the reactor, stirring and heating up to 70-85° C. to carry out reaction;removing the pore-forming agent after the reaction is completed, and screening and collecting the resin with appropriate particle size, and vacuum drying to obtain a porous polymer resin; andcarrying out a further reaction with the resin to obtain a solid-phase synthesis carrier having amino group or carboxyl group.
  • 28. The method according to claim 8, comprising the following steps of: adding 2 L of purified water, 20 g of polyvinyl alcohol and 30 g of sodium chloride into a 3 L reactor equipped with a condenser, an agitator and a thermometer, and dissolving to obtain an aqueous phase;weighing out 108.8 g of styrene, 14 g of 1,2-di (p-vinylphenyl) ethane, 12.2 g of p-chloromethyl styrene, 5 g of fumaronitrile, 6 g of sorbitol trioleate, 40 g of isooctanol, 20 g of isododecane and 2.5 g of benzoyl peroxide, and mixing well to obtain an oil phase;adding the oil phase into the reactor, stirring, and heating up to 80° C. to carry out polymerization for 6 h; washing with hot water after the polymerization is completed, removing the pore-forming agent by ethanol reflux extraction, screening and collecting the resin a particle size of 50-100 μm and vacuum drying to obtain a polymer porous resin with a chlorine content of 565 μmol/g;adding 50 g of the polymer porous resin and 500 ml of N,N-dimethylformamide into a 1 L reactor equipped with a condenser, an agitator and a thermometer, and stirring; then adding 30 g of potassium phthalate and heating up to 95° C. to carry out reaction for 16 hours; cooling to room temperature after the reaction is completed, washing twice with N,N-dimethylformamide, washing to neutral with purified water, washing three times with absolute ethanol, and filtering and drying the resin; adding 200 g of absolute ethanol and 50 g of hydrazine hydrate into the reactor, heating up to 75° C. and reacting for 16 hours; thereafter washing three times with ethanol/purified water solution with a volume ratio of 50:50, washing to neutral with purified water, washing three times with absolute ethanol, and filtering and drying, adding 200 g of absolute ethanol and 50 g of concentrated hydrochloric acid to the reactor, heating up to 60° C. and reacting for 6 h, thereafter cooling to room temperature, washing to neutral with water, and then vacuum drying to obtain a solid-phase synthesis carrier having an amino content of 554 μmol/g and an average pore diameter of 54 nm measured by mercury intrusion method.
  • 29. The method according to claim 8, comprising the following steps of: adding 2 L of purified water, 20 g of polyvinyl alcohol and 30 g of sodium chloride into a 3 L reactor equipped with a condenser, an agitator and a thermometer, and dissolving to obtain an aqueous phase;weighing out 107.7 g of styrene, 12.8 g of 1,2-di (p-vinylphenyl) ethane, 12.5 g of 4-acetoxystyrene, 7 g of fumaronitrile, 10 g of sorbitol trioleate, 42 g of isooctanol, 21 g of isododecane and 2.5 g of benzoyl peroxide, and mixing well to obtain an oil phase;adding the oil phase into the reactor, stirring, and heating up to 78° C. to carry out polymerization for 6 h; washing with hot water after the polymerization is completed, removing the pore-forming agent by ethanol reflux extraction, screening and collecting the resin a particle size of 50-100 μm and vacuum drying to obtain a polymer porous resin;adding 50 g of the polymer porous resin and 300 ml of acetonitrile into a 1 L reactor equipped with a condenser, an agitator and a thermometer, and stirring; then adding 7.5 ml of hydrazine hydrate slowly and reacting for 3 h at room temperature, washing to neutral with water, and then vacuum drying to obtain a solid-phase synthesis carrier having an hydroxyl content of 538 μmol/g and an average pore diameter of 58 nm measured by mercury intrusion method.
  • 30. A method for the solid phase synthesis of oligonucleotides, comprising using the solid-phase synthesis carrier of claim 1.
  • 31. The solid-phase synthesis carrier according to claim 1, wherein the solid-phase synthesis carrier is a copolymer comprising repeating structural units represented by formula (I), formula (II), formula (III), and formula (IV) in its skeleton:
Priority Claims (1)
Number Date Country Kind
2020113575430 Nov 2020 CN national
PCT Information
Filing Document Filing Date Country Kind
PCT/CN2021/077661 2/2/2021 WO