Patent Description:
The present invention relates to the field of biotechnology, and more particularly, to a method for quantitatively co-expressing multiple proteins in vitro and application thereof.

Fluorescent proteins have been widely used in many research fieldsof biology. Fluorescent protein-based molecular probes and labeling methods have become important research tools for studying biological macromolecules or cell functions through dynamic imaging in living cells or in vivo. Since the gene for green fluorescent protein was first cloned from jellyfish in <NUM>, lots of new fluorescent proteins have been cloned from many marine species and new mutants have been obtained from the modification of fluorescent proteins. Those new fluorescent proteins and mutants can"light up"biomolecules or cells, and exhibit the biomolecules activity, thereby helping us reveal the activity law and nature of these molecules or cells. The spectra of the reported fluorescent proteins are distributed throughout the visible region. Those fluorescent proteins are widely used in such areas as gene expression and regulation, protein spatial positioning and transport, protein folding, signal transduction, protease activity analysis, and biomolecular interaction. The discovery and application of the fluorescent proteins provide a powerful research means for the study of modern biology.

Due to the advances in biotechnology, synthetic biologists are able to quickly and reliably transform biological systems and design and produce biological macromolecules, especially to design and produce protein macromolecules with biological functions. In the development of synthetic biology in the past few years, proteins are mainly engineered inside cells with cells as hosts, but it istime-consuming and difficultto engineer inside the cells. This is because the process of cell growth and adaptability is usually inconsistent with the goal of engineering design and the modification of biological components is greatly limiteddue to the complexity of living cell systems, the difficulty of standardization of genetic elements and the barrier created by cell membrane. In front of those limitations, people try to explore new development directions, which promote the development of a new discipline of engineering technology, that is, cell-free synthetic biology. The cell-free synthetic biology involves an emerging technology-- cell-free synthesis system, also known as in vitro synthesis system, comprising in vitro transcription and translation. In the cell-free protein synthesis system, exogenous target mRNA or DNA serve as the template for protein synthesis, and substrates and transcription and translation-related protein factors required for protein synthesis are manually controlled to synthesize the target proteins. The cell-free protein synthesis system eliminates the steps of plasmid construction, transformation, cell culture, cell collection, and fragmentation to synthesize and express proteins. Therefore, it is a fast, time-saving and convenient way to express protein.

Due to the properties of fluorescent proteins, the fluorescent proteins play an important and irreplaceable role in biological research. How to quantitatively co-express multiple proteins in vitro is an important technical problemfacing at present. After research and retrieval of literatures, we did not find any reports of quantitatively co-expressing multiple proteins in the same reaction system using in vitro cell-free protein synthesis technology. After a lot of experiments and researches on the present invention, we find how to quantitatively co-express multiple fluorescent proteins by adjusting the volume or concentration ratio of template DNA. It can be used for high-efficiency fluorescent indicator molecules, the research and development of fluorescently-labeled cells or organisms for various researches or other purposes, and the like.

A method for quantitatively co-expressing multiple proteins in vitro is disclosed in the present invention. In this method, it is possible to quantitatively co-express multiple proteins in the same reaction system according to the concentration and dosage proportional relation of the template (preferably DNA template) of target protein.

According to the first aspect, the present invention provides a method for quantitatively co-expressing multiple proteins in vitro, comprising the steps of:.

Establishing a standard curve of the relationship between concentration of each of standard proteins and respective luminescence value.

In Step (<NUM>), according to the types of multiple target proteins to be co-expressed, a standard protein corresponding to each target protein is provided; each of the multiple target proteins is independently a protein with a luminous function, and the multiple target proteins can be distinguished from each other based on luminescence properties, and can be detected separately "without mutual interference", thus, quantitative detection of each target protein can be achieved.

In particular, the standard protein in Step (<NUM>) is a standard sample of the target proteins. It can be obtained by separation and purification of the target proteins after synthesis thereof, or it is possible to purchase commercially available analytical pure products.

The expression "vectors containing target protein genes" means that the vectors contain encoding sequences of the target proteins, and they can also be referred to as "vectors of the target proteins". For example, "vectors encoding GFP protein" can be simply referred to as "GFP vectors".

In this step, separate vectors containing target protein genes are created to express each of the target proteins respectively. For each of the target proteins, a separate vector containing its encoding sequence is created, and the target proteins are independently expressed in a co-expression system through their respective separate vectors.

The separate vectors containing the target protein genes in Step (<NUM>) are added to an in vitro cell-free protein synthesis system at different concentration ratios for protein synthesis reaction in vitro, that is, incubation reaction, so as to synthesize the multiple target proteins; after a specified reaction time, a luminescence value for each target protein in a reaction solution is obtained; concentration of each target protein product is obtained according to the standard curve shown in Step (<NUM>), and an equation of quantitative relationship between concentration percentage of each target protein product and concentration percentage of a corresponding vector is obtained by fitting; in the in vitro cell-free protein synthesis system, the total concentration of the vectors remains the same.

When the separate vectors containing the target protein genes are addedat different concentration ratios, in the in vitro cell-free protein synthesis system, the total vector concentration during multiple in vitro protein reactions remains the same.

The total vector concentration refers to a sum of the vectors' concentration of all the target proteins in the in vitro cell-free protein synthesis system.

The productconcentration ratio relationship (such as the mass concentration ratiorelationship) of the multiple target proteins to be achieved is set as the target concentration ratio of the multiple target proteins; the concentration and concentration ratio of the vector for each of the multiple target proteins to be expressed are calculated by using the equation established in Step (<NUM>).

According to the required concentration and/or concentration ratio of each target proteinvector obtained in Step (<NUM>), acorresponding amount of the separate vector of each target protein is added to the in vitro cell-free protein synthesis system as described in Step (<NUM>), and the multiple target proteinsco-expressed are obtained after being reacted for the specific period of time defined in Step (<NUM>).

The multiple target proteins are each independently luminescent protein or fusion protein carrying a luminescent label.

When the concentration of each target protein separate vector in each mother solution is the same, the dosage can also be controlled simply by volume or volume ratio. Examples are as follows:
A method for quantitatively co-expressing multiple proteins in vitro, comprising the steps of: (<NUM>) establishing a standard curve: establishing standard curve of protein concentration-luminescence intensity relationship for each co-expressed protein using corresponding standard protein; (<NUM>) creating separate vectors and mother solutions thereof containing each target protein gene for expressing each target protein respectively, wherein the concentration of the separate vectors of each target protein in each mother solution is the same; (<NUM>) establishing an equation of quantitative relationship between concentration percentage of each target protein and volume percentage of a corresponding vector; wherein the separate vectors containing the target protein genes in Step (<NUM>) are added to the in vitro cell-free protein synthesis system at different volume ratios for protein synthesis reaction in vitro; after a specified reaction time, a luminescence value for each target protein in a reaction solution is obtained; the concentration of each target protein product is calculated according to the standard curve shown in Step (<NUM>), and the equation of quantitative relationship between concentration percentage of each target protein and the volume percentage of the corresponding vector is obtained by fitting; in the in vitro cell-free protein synthesis system, the total concentration of the vectors remains the same; (<NUM>) calculating the vector volume, and corresponding volume ratio required for quantitatively co-expressing the multiple proteins; wherein, according to target concentration ratio relationship of the multiple target proteins to be expressed, the volume and volume ratio of the vector required for each of the multiple target proteins to be expressed are calculated by using the equation established in Step (<NUM>); (<NUM>) quantitatively co-expressing the multiple proteins; wherein, according to the required volume and volume ratio for each target protein vector obtained in Step (<NUM>), a corresponding amount of the separate vector of each target protein is added to the in vitro cell-free protein synthesis system as described in Step (<NUM>), and the multiple target proteins co-expressed are obtained after being reacted for the specific period of time defined in Step (<NUM>); wherein the multiple target proteins are each independently luminescent protein or fusion protein carrying a luminescent label.

The in vitro cell-free protein synthesis system comprises at least the components required for protein synthesis except for the template. The in vitro cell-free protein synthesis system may or may not comprise the template. The in vitro cell-free protein synthesis system can also be prepared in a laboratory, or can be a commercially available product.

As one of the preferred embodiments, the in vitro cell-free protein synthesis system comprises:.

Wherein, the yeast cell may be derived from wild-type cells or genetically modified cells.

Wherein, the wording "optional" in components (c) and (d) refers to be dispensable, and components (c)and (d) are each independently dispensable.

In a preferred embodiment, the in vitro cell-free protein synthesis system comprises: yeast cell extract, trihydroxymethylaminomethane (Tris), potassium acetate, magnesium acetate, nucleoside triphosphate mixture (NTPs), amino acid mixture, potassium phosphate, amylase, polyethylene glycol, maltodextrin, etc..

In another preferred embodiment, the in vitro cell-free protein synthesis system provided in the present invention comprises: yeast cell extract, Tris, potassium acetate, magnesium acetate, nucleoside triphosphate mixture (NTPs), amino acid mixture, potassium phosphate, amylase, polyethylene glycol, maltodextrin, fluorescent protein DNA, etc..

In the present invention, the proportion of the yeast cell extract in the in vitrocell-freeprotein synthesis system is not particularly limited. Generally, the content by volume of the yeast cell extract in the in vitrocell-freeprotein synthesis system is in a range of20%-<NUM>%, preferably, in a range of <NUM>%-<NUM>%, more preferably, in a range of <NUM>%-<NUM>%.

Preferably, the luminescence value of each target protein in Step (<NUM>) is not interfered by other proteins at the maximum emission wavelength.

The concentration in the concentration percentage of each target protein in Step (<NUM>) refers to the final concentration of each target protein synthesized in the reaction solution after a period of reactionsince the template is addedin the in vitrocell-freeprotein synthesis system, that is, the concentration of each target protein product. Preferably, the concentration refers to the concentration of each target protein in the reaction solution after the reaction lasts for <NUM>-<NUM> hours.

Preferably, the reaction time in Step (<NUM>) is consistent with the reaction time defined in Step (<NUM>).

More preferably, the vectors in Step (<NUM>) are plasmids containing target protein encoding sequences. That is, the separate vectors containing respective target protein gene are plasmids containing corresponding target protein encoding sequences, respectively.

In another preferred embodiment, the in vitro cell-free protein synthesis system in Step (<NUM>) is one selected from the group consisting of yeast cell-basedin vitro protein synthesis system, Escherichia coli-basedin vitro protein synthesis system, mammal cell-based in vitro protein synthesis system, plant cell-based in vitro protein synthesis system, insect cell-based in vitro protein synthesis system, and combinations thereof.

In another preferred embodiment, the yeast cell is selected from the group consisting of Saccharomyces cerevisiae, Pichia pastoris and Kluyveromyces, and combinations thereof.

In another preferred embodiment,the luminescence value is relative fluorescence unit (RFU) value.

Preferably, when testing a certain protein to be tested among a plurality of proteins, the luminescence value of the protein to be tested is not interfered by other proteins in the solution when the protein is tested under the conditions of the maximum excitation wavelength and the maximum emission wavelength of the proteinand suitable for the use of optical filters.

In some preferred embodiments, the luminescent label is a polyamino acid (having at least <NUM> amino acid units) with luminescent function, and it can be a peptide or a protein.

In another preferred embodiment, the target protein is a luminescent protein. The luminescent proteinis selected from the group consisting of naturalluminescent protein, modified luminescent proteinand fusion protein containing luminescent protein, and combinations thereof.

In another preferred embodiment, the luminescentprotein is a fluorescent protein. The fluorescent protein is selected from the group consisting of natural fluorescent protein, modified fluorescent protein and fusion protein containing fluorescent protein, and combinations thereof.

In another preferred embodiment, the fluorescent protein is red fluorescent protein, orange fluorescent protein, yellow fluorescent protein, green fluorescent protein, cyan fluorescent protein, blue fluorescent protein or purple fluorescent protein.

In another preferred embodiment, the method for quantitatively co-expressing multiple proteins in vitro further comprises separation and/or purification of the target proteins, that is, it comprises at least one of the following processes: isolation of the target proteins, and purification of the target proteins.

According to the second aspect, the present invention provides a use of the in vitro cell-free protein synthesis system in the method of quantitatively co-expressing multiple proteins in vitro according to the first aspect of the invention.

According to the third aspect, the presentinvention providesone or a plurality of fluorescent proteins expressed by using the in vitro cell-free protein synthesis system. Wherein, the plurality of fluorescent proteins are co-expressed in the same reaction system.

The main advantages of the present invention include:.

As used herein, "in vitro protein synthesis system", "in vitro cell-free protein synthesis system", "cell-free protein synthesis system" have the same meaning and can be used interchangeably.

As used herein, the term "gene" refers to a nucleotide sequence encoding a certain protein. The term "gene" comprises the coding sequence (CDS) of the protein.

The coding sequence is abbreviated as CDS. The nucleotide sequence completely corresponding to the codon of the protein, and the sequence does not contain other sequences not corresponding to the protein (sequence changes during the process of mRNA processing and other processes are not considered).

As used herein, the expression "having a luminous function" refers to have photosensitivity and it allows to emit light of a detectable wavelength. According to luminescence properties, the emitted light herein include but are not limited to fluorescence, phosphorescence, ultraviolet light, infrared light, and the like. According to the principle of luminescence, the luminous function can be photoluminescence, chemiluminescence, self-luminescence, etc..

In the present invention, the characterization method of substance concentration is not particularly limited, as long as quantification can be achieved by using the following methods, including but not limited to mass concentration, molar concentration, mass volume concentration and volume concentration. For proteins, vectors and other substances, a concentration form suitable for characterization and quantification can be independently used.

As used herein, "concentration of target protein" is preferablymass concentration or mass volume concentration, and other quantifiable concentration forms, such as molar concentration, can also be selected.

As used herein, "multiple" means two or more.

As used herein, "multiple times" means twice or more.

As used herein, "optional" means that it is not necessarily an embodiment of the present invention, but it can be selectively applied depending on the technical solutions of the present invention. Andwhether it is suitable for the technical solutions of the invention is taken as the selection basis.

As used herein, "combinations thereof" means any suitable combinations, including at least two objects listed above.

It should be understood that the above-mentioned technical features of the present invention and the technical features specifically described hereinafter (such as in Examples) can be combined with each other to form a new or preferred technical solution.

In some preferred embodiments, the invention provides an in vitro protein synthesis system, comprising:.

The wording "optional" incomponents (c) and (d) each independently represents the components (c) and (d) are dispensable.

In a preferred embodiment, the in vitro protein synthesis system according to the present invention comprises yeast cell extract, Tris, potassium acetate, magnesium acetate, nucleoside triphosphate mixture (NTPs), amino acid mixture, potassium phosphate, amylase, polyethylene glycol, maltodextrin, etc. Fluorescent protein DNA and other substances can be further added to the in vitro protein synthesis system for in vitro protein synthesis reactions.

In the present invention, the cell extract preferably does not contain intact cells. Suitable reported cell extract preparation techniques can be selected to prepare the cell extract. The preparation of the cell extract usually comprises at least the following steps of: providing an appropriate amount of yeast cells, breaking the cells, performing solid-liquid separation, and collecting the supernatant. The extraction product obtained according to the preparation method of the cell extract may have a small or very small amount of intact cells left, and this type of extraction product also falls within the scope of the cell extract of the present invention. The cell extract does not exclude the presence of intact cells.

The in vitro protein synthesis system of the present invention also does not exclude the existence of intact cells as long as it does not affect the realization of the purpose of the present invention, that is, it does not affect the realization ofquantitative co-expression. There are many factors behind the presence of those intact cells. The intact cells may be residues caused by the process of preparing the cell extract, or they may be introduced intentionally, for example, the cell fragments obtained by simple fragmentation of cells added may be a mixture of the completely fragmented product and the intact cells; or the intact cellsare present due to the addition of intact cells alone.

Typical cell extract (including yeast cell extract) comprises ribosome, tRNA and aminoacyl tRNAsynthetasefor protein translation, initiation factors, elongation factors and termination release factors required for protein synthesis. Furthermore, the cell extract (including yeast cell extract)also comprises some other proteins derived from the cytoplasm, especially soluble proteins.

In some preferred embodiments, the yeast cell extract is Kluyveromyces cell extract. In some preferred embodiments, the Kluyveromyces is selected from the group consisting of Kluyveromyceslactis(K. lactis), Kluyveromyceslactis var. drosophilarum, Kluyveromyceslactis var. lactis,Kluyveromycesmarxianus,Kluyveromycesmarxianus var. lactis,Kluyveromycesmarxianus var. marxianus,Kluyveromycesmarxianus var. vanudenii, Kluyveromycesdobzhanskii,Kluyveromycesaestuarii,Kluyveromycesnonfer mentans,Kluyveromyceswickerhamii,Kluyveromycesthermotolerans,Kluyv eromycesfragilis,Kluyveromyceshubeiensis,Kluyveromycespolysporus,Klu yveromycessiamensis,Kluyveromycesyarrowii, and combinations thereof.

The protein components (e.g., RNApolymerase)required in the in vitro cell-free protein synthesis system can be provided endogenously or be added exogenously. When they are provided endogenously, it is allowed to refer to genetic modification methods provided in the following existing documents and cited documents, including but not limited to: <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>,"<NPL>". Those methods comprise inserting the coding sequences into an intracellular episomal plasmid, integrating the coding gene into the cell genome, or a combination thereof. When they are provided exogenously, their content can be controlled and adjusted as required by the system.

In some preferred embodiments, the in vitro cell-free protein synthesis system comprises:yeast cell extract, Tris, potassium acetate, magnesium acetate, nucleoside triphosphate mixture (NTPs), amino acid mixture, potassium phosphate,sugar (any one of glucose, sucrose, maltodextrin and combinations thereof, and when maltodextrin is contained, amylase is also preferably contained), polyethylene glycol, RNA polymerase, etc. The RNA polymerase can be provided endogenously or added exogenously. One of the more preferred forms of the RNA polymerase is T7 RNA polymerase.

In some preferred embodiments, the in vitro cell-free protein synthesis system comprises exogenously added RNA polymerase.

In some preferred embodiments, the in vitro cell-free protein synthesis system comprises exogenously added T7 RNA polymerase.

In some preferred embodiments, the in vitro cell-free protein synthesis system comprises Kluyveromyceslactis cell extract and exogenously added T7 RNA polymerase. In some preferred embodiments, the concentration of the T7 RNA polymerase is in a range of <NUM>-<NUM>/mL. In some other preferred embodiments, the concentration of the T7 RNA polymerase is in a range of <NUM>-<NUM>/mL. In some other preferred embodiments, the concentration of the T7 RNA polymerase is in a range of <NUM>-<NUM>/mL. In some other preferred embodiments, the concentration of the T7 RNA polymerase is <NUM>/mL.

In the present invention, the protein content of the yeast cell extract ispreferably in a range of20mg/mL-<NUM>/mL, more preferably in a range of <NUM>/mL-<NUM>/mL. The method for measuring the protein content isCoomassie brilliant blue assay.

The mixture of nucleoside triphosphates in the in vitro cell-freeprotein synthesis system preferablycomprises adenosine triphosphate, guanosine triphosphate, cytidine triphosphate and uridine triphosphate. In the present invention, there is no limitation to the concentration of various mononucleotides. Generally, the concentration of each mononucleotide is in a range from <NUM> to <NUM>, preferably in a range from <NUM> to <NUM>.

The amino acid mixture in the in vitrocell-free protein synthesis system may comprise natural or unnatural amino acids, and may include amino acidsof D-type or amino acids of L-type. Representative amino acids include, but are not limited to, <NUM> types of natural amino acids including: glycine, alanine, valine, leucine, isoleucine, phenylalanine, proline, tryptophan, serine, tyrosine, cysteine, methionine, asparagine, glutamine, threonine, aspartic acid, glutamic acid, lysine, arginine and histidine. The concentration of each amino acid is usually in a range from <NUM> to <NUM>, preferably, in a range from <NUM> to <NUM>, such as <NUM>, <NUM>, <NUM> and <NUM>.

In some preferred embodiments, the in vitro cell-free protein synthesis system further comprises polyethylene glycol (PEG) or analogs thereof. The concentration of polyethylene glycol or analogs thereof is not particularly limited. Generally, the concentration (w/v) of polyethylene glycol or analogs thereof is in a range from <NUM>% to <NUM>%, preferably, in a range from <NUM>% to <NUM>%, more preferably, in a range from <NUM>% to <NUM>%, based on the total volume of the protein synthesis system. Representative examples of PEG include, but are not limited to, PEG3000, PEG8000, PEG6000 and PEG3350. It should be understood that the system according to the present invention may further comprise polyethylene glycol with other various molecular weights (such as PEG <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM>, <NUM> and so on).

In some preferred embodiments, the in vitro cell-free protein synthesis system further comprises sucrose. The concentration of sucrose is not particularly limited. Generally, the concentration(w/v) of sucrose is in a range from <NUM>% to <NUM>%, preferably, in a range from <NUM>% to4%, more preferably, in a range from <NUM>% to <NUM>%, based on the total volume of the protein synthesis system.

In addition to the yeast extract, some particularly preferred in vitrocell-free protein synthesis systems further comprise the following components: <NUM> mMTris (pH <NUM>), <NUM>-<NUM> potassium acetate, <NUM>-<NUM> magnesium acetate, <NUM>-<NUM> nucleoside triphosphate mixture, <NUM>-<NUM> amino acid mixture, <NUM>-<NUM> mMpotassium phosphate, <NUM>-<NUM>/mL amylase, <NUM>%-<NUM>% polyethylene glycol, <NUM>-<NUM> maltodextrin (based on the molar amount of glucose unit), <NUM>-<NUM> ng/µL fluorescent protein DNA, etc. Furthermore, the total volume of the in vitrocell-free protein synthesis system is in a range from <NUM>µL to <NUM>µL, preferably, in a range from <NUM>µL to <NUM> uL, preferably <NUM>µL. The yeast extract is more preferably Kluyveromyces cell extract, and more preferably Kluyveromyceslactiscell extract.

In addition to the yeast extract, someparticularly preferred in vitrocell-free protein synthesis systems further comprise the following components: <NUM> mMTris (pH <NUM>), <NUM>-<NUM> potassium acetate, <NUM>-<NUM> magnesium acetate, <NUM>-<NUM> nucleoside triphosphate mixture, <NUM>-<NUM> amino acid mixture, <NUM>-<NUM> mMpotassium phosphate, <NUM>-<NUM>/mL amylase, <NUM>%-<NUM>% polyethylene glycol, <NUM>-<NUM> maltodextrin(based on the molar amount of glucose unit), <NUM>-<NUM>/mL T7 RNA polymerase, etc. Those components can be mixed with <NUM>-<NUM> ng/µL fluorescent protein DNA for in vitro protein synthesis reaction. The reaction volume is preferably in a range from <NUM>µL to <NUM>µL. One of the preferred volumes is <NUM>µL.

In the present invention, the term "template"refers to a nucleic acid template used to direct protein synthesis, which can be mRNA, DNA templateor a combination thereof, and it is preferably a DNA template. It can be linear or circular, and one of the preferred templates is a circular plasmid.

During the process of in vitro protein synthesis, the promoter in the template for initiating the synthesis of target protein can be selected from the group consisting of AOD1, MOX, AUG1, AOX1, GAP, FLD1, PEX8, YPT1, LAC4 , PGK, ADH4, AMY1, GAM1, XYL1, XPR2, TEF, RPS7, T7 and any suitable combinations thereof. One of the preferred promoters is T7 promoter.

In the present invention, no mutual interference means that when testingone or more proteins to be tested (i.e., target proteins) in a plurality of proteins are measured in a mixed solution containing a plurality of proteins, the luminescence value of other fluorescent proteins or fusion proteins has little or no overlap with the luminescence value of one or more proteins to be tested under the luminescence detection conditions of the experiment, such as, the conditions of the maximum excitation wavelength, the maximum emission wavelength and suitable for the use of optical filters. It should be noted that if the optical filters used do not match the optical properties of the proteins, it may lead to inaccurate characterization of some linear relationships, such as the linear relationship between the protein ratio and the percentage of the corresponding vector in the following embodiments.

It should be noted that under the fluorescence detection conditions of this experiment, if the luminescence values of other fluorescent proteins or fluorescent fusion proteins have a partial overlap with(i.e., interfere with) the luminescence value of one or more proteins to be tested, thetechnical solution in the present inventioncan be implemented. The partial overlap means that under certain fluorescent detection conditions, the measured luminescence signal comprises luminescence signals of proteins to be tested and of other proteins, and such an overlap does not affect the detection of theproteins to be tested by using the technical solution of the present invention.

In the present invention, standard proteins refer to protein samples for calibrating the linear relationship between the concentration of one or more target proteins and the luminescence values. The standard proteins can be fluorescent proteins or fluorescent fusion proteins, which are determined according to the light-emitting unit contained in the target protein molecule to be tested. For example, the standard proteins can be the target proteins or the fluorescent proteins (when the target proteins are fusion fluorescent proteins, it means that the target protein molecules are fused withfluorescent proteins) contained in the structure of the target proteins, or luminescent labels. The purity and concentration of the standard protein samples are known or determined before use.

In the present invention, such a process refers to one in which the product concentration of the multiple proteins in a reaction system is assigned a specific ratio, and the in vitro protein synthesis reaction is initiated at this preset concentration ratio, so that products of the multiple target proteins with preset concentration proportion relationship can be obtained; or, the product concentration of the multiple target proteins in the reaction system is assigned a specific value, and the in vitro protein synthesis reaction is initiated at this concentration, so that products of the multiple proteins with desired quantitative relationship can be obtained.

Shimomura isolated green fluorescent protein (GFP) from jellyfish for the first time, and Chalfie cloned GFP into other species for expression for the first time. Tsien took the lead in elaborating the chemical mechanism of GFP luminescence, and obtained a GFP mutant (GFP-S65T) with greatly enhanced fluorescence intensity and light stability through single point mutation (S65T) technology. Many scientists, represented by Tsien, introduced genetic mutations into GFP to further transform GFP to obtain blue fluorescent protein (BFP, blue FP), cyan fluorescent protein (CFP, Cyan FP), green fluorescent protein (GFP, green FP) and yellow fluorescent protein (YFP, yellow FP). Later, researchers cloned red-shifted fluorescent proteins from corals, sea anemones and other species,which greatly expanded the multicolor imaging applications of fluorescent proteins. In recent years, scientists have skillfully applied light-activated and light-converted fluorescent proteins to high-resolution imaging, breaking the optical diffraction limit and having a resolution of tens of nanometers. It is a revolutionary leap in the history of microscopic imaging technology. Since then, fluorescent proteinshave become a driver for the further development of life science.

In <NUM>, Qsamu Shimomura first discovered green fluorescent protein (GFP) in Aequorea Victoria, a jellyfish living in the icy waters of the Arctic Ocean, and isolated and purified GFP. Martin Chalfie discovered the values of GFP, and carried out an experimental research by using GFP, a magic tool for the first time. In <NUM>, YongjianQian modified GFP, which made the fluorescence of GFP become stronger and change color. Those three scientists won the Nobel Prize in Chemistry in <NUM>. Since then, fluorescent proteinshaveled to a new revolution in biotechnology. The GFP found in jellyfish is composed of <NUM> amino acids with a molecular weight of <NUM>. 9kDa, and amino acids at positions <NUM>, <NUM>, and <NUM> spontaneously form a fluorescent luminescent group --p-hydroxybenzyl imidazolidinone, which can be excited by light to produce fluorescence. Many scientists used the luminescence mechanism of fluorescent proteins to extract the fluorescent protein gene from jellyfish and transfer it to other organisms, making biological changes more diversified. Since GFP was cloned in <NUM>, scientific researchers have designed many GFP mutants and non-mutant proteins, providing powerful research means for modern biological research.

Since the fluorescent proteins have a variety of colors, and their fluorescence is stable and non-toxic, they can develop colors without addition of substrates and cofactors, which are not limited by species, cell types and locations, and the fluorescent proteins can make the complex system structure visualized and can be detected at regular time and at specific positions, so the fluorescent proteins have been widely used. The reported fluorescent protein spectra are distributed throughout the visible region and are widely used in biological research fields such as gene expression and regulation, protein spatial positioning and transport, protein folding, signal transduction, protease activity analysis, and biomolecular interaction, so there emerge fluorescent mice, fluorescent rabbits, and fluorescent pigs. In the meantime, they are also used in the fields of tumor pathogenesis, drug screening, feed material improvement, aquatic environment detection and nutrition metabolism research, etc..

In the present invention, with consideration of practical use,proteins with different excitation and emission wavelengths, high brightness, different aggregate structures and different colors are selected. A total of <NUM> types of <NUM> proteins having the following mutants (proteins modified based on eGFP) characteristics shown in Table <NUM> are selected.

An reported in vitro cell-free protein synthesis system, based on the following cell types of Escherichia coli, wheat germ cell, rabbit reticulocyte lysate (RRL), Saccharomyces cerevisiae, Pichia pastoris, Kluyveromycesmarxianus and other cell types, can be incorporated into the present invention as an alternative form of the in vitro protein synthesis system of the present invention. For example, Escherichia coli-based in vitro cell-free protein synthesis system recorded in <CIT>, and the in vitro cell-free protein synthesis system recorded in the cited document in sections, including but not limited to "<NPL>. <NPL>", can be used to implement thein vitro protein synthesis system of the present invention when appropriate.

The in vitro protein synthesis system, templates, plasmids, target proteins, in vitro protein synthesis reaction (incubation reaction), various preparation methods, various detection methods and other technical elements of the present invention can independently obtain suitable implementation methods from the following documents, including but not limited to: <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>(<CIT>), <CIT>(<CIT>), <CIT>(<CIT>), <CIT>(<CIT>), <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>, <CIT>. Unless they conflict with the purposes of the present invention, these documents and their cited documents are cited herein in their entirety.

The present invention further discloses amethod for quantitatively co-expressing multiple proteins in vitro, comprising the steps of:.

Under the guidance of the present invention, a method for quantitatively co-expressing the multiple proteins by quantitatively determining the expression level of a protein product in a non-fluorescent manner or a non-luminescent manner is also within the scope of the present invention. The protein expression level is quantitatively characterized by the non-luminescent manner, such as ultraviolet absorption and infrared absorption.

The present invention is further described below in conjunction with specific examples and the accompanying <FIG>. The technical flow of the process used in Examples <NUM>-<NUM> is shown in <FIG>. It should be understood that these examples are only used to illustrate the present invention and not to limit the scope of the present invention. With respect to the experimental methods without specifically described conditions in the following examples,one person may generally follow conventional conditions, such as the conditions described in <NPL>), or follow the conditions recommended by the manufacturer. Unless otherwise stated, percentages and portionsrefer to percentages and portions by weight. In the following examples, Kluyveromyceslactis(Kluyveromyceslactis NRRL Y-<NUM>) is only an example for illustration, and it does not imply that the present invention is only applied to Kluyveromyceslactis, instead, it is only used as a specific expression system of the present invention for research; the technical solution in the examples is also applied to other yeast cell-basedin vitro protein synthesis system, Escherichia coli-basedin vitro protein synthesis system, mammal cell-based in vitro protein synthesis system, plant cell-based in vitro protein synthesis system, insect cell-based in vitro protein synthesis system.

Unless otherwise specified, materials and reagents used in the examples of the present invention are all commercially available products.

By searching different databases, the coding sequences of <NUM> different fluorescent protein genes were subjected to Blast, and the codons were optimized to make them suitable for Kluyveromyceslactis-based in vitro cell-free protein synthesis system.

The optimized DNA sequences in Table <NUM> were used for genome synthesis.

Primer designing was performed by Oligo <NUM> software, and sequences of primers are shown in Table <NUM>.

Inserting gene sequences of target proteins to be expressed into pD2P plasmids (see <FIG>), and construction processof plasmids is as follows:
With pD2P plasmid as template, construction of plasmids was carried out by using molecular cloning techniques. Two PCR amplification processes were carried out by using two pairs of primers, respectively. <NUM>µL product of each PCR amplification process were mixed followed by the addition of 1µL of DpnIand <NUM>µL of <NUM> × Cutsmart buffer, and then the mixture was incubated at <NUM> for <NUM> hours. <NUM>µL of DpnI-treated productwas added into <NUM>µL of DH5α competent cells. The mixture was placed on ice for <NUM> minutes, heat-shocked at <NUM> for <NUM> seconds, followed by the addition of <NUM> of LB liquid medium, and then cultured with shaking at <NUM> for <NUM> hour. Thereafter, the mixture was coated onto an Amp-resistant LB solid medium, and then an inverted culture was carried out at <NUM> until monoclonal colonies grew out. Three monoclonal colonies were picked out and then cultured for expansion. After it was confirmed to be correct by sequencing, the plasmids were extracted and stored, and the plasmid concentration was adjusted to the same level. Before use, all plasmids were measured based on OD values, and the concentration was adjusted to the same concentration (450ng/µL), that is, the concentration of the mother solution of the template/vector of each target protein is the same.

The coding gene of the target protein in the pD2P plasmid was initiated with a T7 promoter.

All the fragments between the transcription initiation sequence <NUM>' UTR and termination sequence <NUM>' UTR in all the plasmids were amplified with the above-mentioned plasmid as template by using random seven-base primers according to a method for performing amplification process using phi29 DNA polymerase. The amplified products were used as DNA templates for synthesis of various fluorescent proteins. One or more tandem combinations were included between the transcription initiation sequence <NUM>' UTR and terminationsequence <NUM>' UTR. The tandem combination comprises translation-enhancing regulatory elements and protein expression and purification tag elements.

According to the instruction, the prepared DNA templates of the fluorescent proteins (the mother solution concentration of the templates of different fluorescent proteins was the same) were added to self-made Kluyveromyceslactis-based in vitro cell-free protein synthesis system.

The in vitrocell-free protein synthesis system (having a total volume of <NUM>µL) used in the example comprises:Kluyveromyceslactiscell extract <NUM>% (v/v), <NUM> mMTris (pH <NUM>), <NUM> potassium acetate, <NUM> magnesium acetate, <NUM> nucleoside triphosphate mixture, <NUM> amino acid mixture, <NUM> mMpotassium phosphate, <NUM>/mL amylase, <NUM>% (w/v)polyethylene glycol (PEG-<NUM>), <NUM> maltodextrin(in glucose unit, equivalent to about <NUM>/mL), <NUM>/mL exogenously added RNA polymerase, and <NUM> ng/µL fluorescent protein DNA, etc. When the type of fluorescent protein DNA is greater than <NUM>, 15ng/µL here is the total concentration of all the fluorescent protein DNA.

The above-mentioned reaction system was placed in an environment at <NUM>-<NUM>, and was incubated for about <NUM> hours. During the reaction process, different fluorescence may be observed and color of the fluorescence gradually looked darker during a certainperiod of time. After the reaction was completed, the reaction system was immediately placed on the Tecan Infinite F200/M200 multifunctional microplate reader. Different optical filters were selected, and corresponding maximum excitation and emission wavelengths were set according to characteristics of the fluorescent proteins to be measured, the value was read, the strength of each fluorescence signal was detected, and the Relative Fluorescence Unit (RFU) value was taken as an active unit, and the results were shown in <FIG>.

The fluorescent proteins obtained by the reaction wereoptimized and purified by commercially available nickel beads (Sangon, C600033). Please refer to the instructions for the specific purification method. The purity of the purified protein sample was determined to obtain its protein concentration. The purified protein was made into solution. 1µL <NUM>×SDS-loading buffer (without DTT) was added to <NUM>µL of the solution for SDS-PAGE; then fluorescence imaging was performed. Several proteins with obvious fluorescence were selected as examples, as shown in <FIG>(<FIG> and <FIG>). 10µL of the above purified protein was taken out, and <NUM>µL <NUM>×SDS-loading buffer ( containing <NUM> DTT) was added to <NUM>µL of the purified protein for SDS-PAGE; Coomassie brilliant blue staining, decolorization and gel imaging were performed sequentially; wherein results before optimization were shown in <FIG>(<FIG> and <FIG>), results after optimization were shown in <FIG>(<FIG> and <FIG>).

The protein sample purified by nickel beads in Example <NUM> was used as the standard protein sample. The protein sample was diluted with buffer (500mMNaCl+20mMTris-HCl (pH8. <NUM>)) in different gradients way, and the protein of different concentrations was placed on the Tecan Infinite F200/M200 multifunctional microplate reader. Different optical filters were selected, and corresponding maximum excitation and emission wavelengths were set according to characteristics of the fluorescent proteins to be measured, and RFU value was read. The fluorescent proteins tdTomato, clover and Micy were taken as examples, and the concentration of a single protein was positively correlated with RFU value, as shown in <FIG> (6a-6d). The protein mass concentration standard curves were obtained by fitting the curve by plotting the signal strength against the protein concentration, wherein the protein mass concentration standard curves were as follows: <MAT> <MAT> <MAT>.

In the formulas, y<NUM>,y<NUM> and y<NUM> represent the mass concentration (unit: µg/mL) of the proteins tdTomato, Clover and Micy to be tested, respectively; and X<NUM>, X<NUM>, and X<NUM>represent the luminescence values (RFU) of tdTomato, Clover, and Micy, respectively.

<NUM>) Detecting the relationship between the template ratio and the relative fluorescence unit (RFU)value when a single protein was expressed. The prepared DNA templates of the fluorescent proteins (the mother solution concentration of the templates of different fluorescent proteins was the same) were added to self-made Kluyveromyceslactis-based in vitro cell-free protein synthesis system.

The in vitrocell-free protein synthesis system (having a total volume of <NUM>µL) used in the example comprises: Kluyveromyceslactiscell extract <NUM>% (v/v), <NUM> mMTris (pH <NUM>), <NUM> potassium acetate, <NUM> magnesium acetate, <NUM> nucleoside triphosphate mixture, <NUM> amino acid mixture, <NUM> mMpotassium phosphate, <NUM>/mL amylase, <NUM>% (w/v) polyethylene glycol, <NUM> maltodextrin (in glucose unit, equivalent to about <NUM>/mL), and <NUM> ng/µL fluorescent protein DNA, etc..

The above-mentioned reaction system was placed in an environment at <NUM>-<NUM>, and was incubated for about <NUM> hours. After the reaction was completed, the reaction system was immediately placed on the Tecan Infinite F200/M200 multifunctional microplate reader. Corresponding maximum excitation and emission wavelengths were set according to characteristics of the fluorescent proteins tested, and RFU value was read. The fluorescent proteinstdTomato, Clover, and Micy were taken as examples. When tdTomato, Clover, or MiCy are expressed separately, the protein yield was independent of the amount of template (1µL template per 30µL system), as shown in <FIG> (7a-7c).

Detecting the relationship betweenthe volume percentage (i.e., percentage obtained relative to the total amount of the template DNA of the two fluorescent proteins) of the template NDA of a protein in a system where two proteins were co-expressed and the percentage of the amount of the protein mass (i.e.,the ratio of each target protein mass in the total target protein mass, in percentage). The volume percentage of each protein template here was consistent with the concentration percentage of each protein.

The prepared DNA templates of the fluorescent proteins (the mother solution concentration of the templates of different fluorescent proteins was the same) were added to self-made Kluyveromyceslactis-based in vitro cell-free protein synthesis system.

The in vitrocell-free protein synthesis system (having a total volume of <NUM>µL) used in the example comprises: Kluyveromyceslactiscell extract <NUM>% (v/v), <NUM> mMTris (pH <NUM>), <NUM> potassium acetate, <NUM> magnesium acetate, <NUM> nucleoside triphosphate mixture, <NUM> amino acid mixture, <NUM> mMpotassium phosphate, <NUM>/mL amylase, <NUM>% (w/v)polyethylene glycol,<NUM> maltodextrin(in glucose unit, equivalent to about <NUM>/mL), and <NUM> ng/µL fluorescent protein DNA (equivalent to the total concentration of the template), wherein the total volume of the two fluorescent proteins was 1µL.

The above-mentioned reaction system was placed in an environment at <NUM>-<NUM>, and was incubated for about <NUM> hours. After the reaction was completed, the reaction system was immediately placed on the Tecan Infinite F200/M200 multifunctional microplate reader. Corresponding maximum excitation and emission wavelengths were set according to characteristics of the fluorescent proteinstested, and RFU value was read. When two proteins are co-expressed, for example, when tdTomatoandClover, or tdTomato and MiCy are co-expressed in the same reaction system, it was found that the protein yield was positively correlated with the amount of the template, and the relationshipwas substantially linear, as shown in <FIG> (8a-8d). In <FIG>, co-expression of tdTomato and Clover was taken as an example to show that the linear relationship between the proportion of a single protein and the percentage of its vector; in addition, the co-expression of tdTomato and MiCy also showed a similarlinear relationship between the proportion of a protein and the percentage of a corresponding vector.

Creating a standard curve by plotting the volume percentage of the template DNA (i.e., the ratio of a certain template volume to the total template volume, which is numerically equal to the ratio of a certain template concentration to the total template concentration) against the obtained concentration percentage of the protein (i.e., the ratio of each protein in the total system to the total protein) as follows, with the co-expression of tdTomato and Clover as an example, by combining the standard curve of Example <NUM>.

When tdTomato and Clover were co-expressed, <MAT> <MAT>.

In the formulas, y<NUM> and y<NUM> represent the percentage of proteins tdTomato, Clover, x<NUM>represents the volume percentage of the template DNA of tdTomato when two proteins are co-expressed.

Detecting the relationship between the template ratio of a single protein in a system where three proteins were co-expressed and the relative fluorescence unit (RFU) value.

The in vitrocell-free protein synthesis system (having a total volume of <NUM>µL) used in the example comprises: Kluyveromyceslactiscell extract <NUM>% (v/v), <NUM> mMTris (pH <NUM>), <NUM> potassium acetate, <NUM> magnesium acetate, <NUM> nucleoside triphosphate mixture, <NUM> amino acid mixture, <NUM> mMpotassium phosphate, <NUM>/mL amylase, <NUM>% (w/v)polyethylene glycol,<NUM> maltodextrin(in glucose unit, equivalent to about <NUM>/mL), and <NUM> ng/µL fluorescent protein DNA (equivalent to the total concentration of the template), wherein the total volume of the three fluorescent proteins was 1µL.

The above-mentioned reaction system was placed in an environment at <NUM>-<NUM>, and was incubated for about <NUM> hours. After the reaction was completed, the reaction system was immediately placed on the Tecan Infinite F200/M200 multifunctional microplate reader. Corresponding maximum excitation and emission wavelengths were set according to characteristics of the fluorescent proteinstested, and RFU value was read. When three proteins, for example, tdTomato, Clover, and mKate1. <NUM> were co-expressed; and when tdTomato, Clover, and mNeptune2 were co-expressed, it appeared to be a linear relationship similar to that shown in the previous example (i.e., Example <NUM>), that is, protein yield was positively correlated with the amount of the template, and the relationship was substantially linear. A1, B1, C1, D1, E1, F1, G1 represent Clover:tdTomato:mKate1. <NUM> template ratio were1:<NUM>:<NUM>, <NUM>:<NUM>:<NUM>, <NUM>:<NUM>:<NUM>, <NUM>:<NUM>:<NUM>, <NUM> :<NUM>:<NUM>, <NUM>:<NUM>:<NUM>, <NUM>:<NUM>:<NUM>, respectively; and A2, B2, C2, D2, E2, F2, G2 represent Clover:tdTomato:mNeptune2template ratio were <NUM>:<NUM>:<NUM>, <NUM>:<NUM>:<NUM>, <NUM>:<NUM>:<NUM>, <NUM>:<NUM>:<NUM>, <NUM>:<NUM>:<NUM>, <NUM>:<NUM>:<NUM>, respectively, as shown in <FIG> (9a-9d).

The protein percentage standard curves fitted by the template ratio and the protein yield ratioin this example were as follows:
When tdTomato, Clover and mKate1. <NUM> were co-expressed, <MAT>.

In the formula, y<NUM> is the content of the protein Clover to be measured (relative to the total amount of all the proteins), x<NUM> is the volume percentage of the template DNA of Clover when three proteins are co-expressed.

When tdTomato, Clover and mNeptune2were co-expressed, <MAT>.

In the <FIG>, only Clover was taken as an example to show that the linear relationship between the proportion of its protein and the percentage of its vector; in addition, the other two proteins co-expressed also showed a similar linear relationship between the proportion of a protein and the percentage of a corresponding vector.

The mass concentration ratio of the two target proteins synthesized was <NUM>:<NUM> as required, that is, the concentration of the tdTomato protein is <NUM>%,and the concentration of the Micy protein was <NUM>%. The volume ratio relationship (consistent with the concentration ratio relationship)of the template DNA of the two fluorescent proteins was calculated according to the equation obtained in Example <NUM> when tdTomato and Clover were co-expressed: <MAT>.

In the formula, y represents the percentage of tdTomato protein, <NUM>-y<NUM>represents the percentage of Clover protein, and x<NUM> is the volume percentage of tdTomato template DNA when the two proteins are co-expressed.

That is to say, when y<NUM>was <NUM>%, it was calculated that x<NUM>=<NUM>%/<NUM>=<NUM>%, <NUM>-x<NUM>=<NUM>-<NUM>%=<NUM>%, that is, the volume ratio of the vectors of the two proteins tdTomato and Clover was <NUM>:<NUM>. When the total volume of the two protein vectorswas 1µL, the volume of the tdTomato vector added therein was0. <NUM> pL, and the volume of the Clover vector added therein was <NUM>µL.

According to the above calculation results,<NUM>. 48µL and <NUM>. 52µL of DNA templates (450ng/µL) of the two fluorescent proteins, tdTomato and Clover, having the same template mother solution concentration, were added to self-made Kluyveromyceslactis-based in vitro cell-free protein synthesis system (having a total volume of 30µL). Wherein the in vitro cell-free protein synthesis system comprises Kluyveromyceslactis cell extract <NUM>% (v/v), <NUM> mMTris (pH <NUM>), <NUM> potassium acetate, <NUM> magnesium acetate, <NUM> nucleoside triphosphate mixture, <NUM> amino acid mixture, <NUM> mMpotassium phosphate, <NUM>/mL amylase, <NUM>% (w/v)polyethylene glycol,<NUM> maltodextrin(in glucose unit, equivalent to about <NUM>/mL), and <NUM> ng/µL fluorescent protein DNA (equivalent to the total concentration of the template), wherein the total volume of templates of the two fluorescent proteins, tdTomato and Clover was <NUM>µL.

The above-mentioned reaction system was placed in an environment at <NUM>-<NUM>, and was incubated for about <NUM> hours. After the reaction was completed, the reaction system was immediately placed on the Tecan Infinite F200/M200 multifunctional microplate reader. Corresponding maximum excitation and emission wavelengths were set according to characteristics of the fluorescent proteinstested, and RFU value was read. RFU values of tdTomato and Clover were <NUM> and <NUM>, respectively. Substituting the obtained RFU values into the standard curve relational expression described in Example <NUM>: <MAT> <MAT>.

In the formulas, y<NUM> andy<NUM> represent the mass concentration (unit: µg/mL) of the proteins tdTomatoand Clover to be measured, respectively;and X<NUM>, X<NUM>represent the luminescence values (RFU) of tdTomato and Clover. It can be obtained from the above formulas that the mass concentration of tdTomato and Clover to be tested were <NUM>. 64µg/mL and <NUM>. 22µg/mL, respectively, and that the ratio of the mass concentrations of the two proteins was42. <NUM>:<NUM>, similar to <NUM>:<NUM>. Such results were substantially the same as we had expected. As a result, the method of the present invention is accurate and feasible for quantitatively co-expressing multiple proteins in vitro.

For the first time, the invention provides a method for quantitatively co-expressing multiple proteins in vitro. In this method, the multiple proteins are synthesized by using an in vitro cell-free protein synthesis system, which is simple, efficient and fast. When it is used to synthesize fluorescent proteins, measurable fluorescence intensity, which is visually detectable with naked eyes, can be generated. Compared with conventional methods, it can monitor expression proteins in real time in an efficient and intuitive manner, and it allows complex phenomenon to be simplified. A method for quantitatively co-expressing multiple fluorescent proteins, that is, a method for simultaneously synthesizing multiple proteins in the same system, is provided. In this method, according to the preset ratio (target ratio), the multiple target proteins can be synthesized quantitatively at thetarget ratio.

The above descriptions are only part of embodiments of the present invention;the invention is not limited to those embodiments. Under the guidance and teachings of the technical solution of the present invention, many modifications and variations having the same technical effects will be apparent to those of ordinary sill in the art and are within the scope of the present invention.

All documents mentioned in the present invention are cited as references in this application, just as each document is individually cited as a reference. Additionally, it should be understood that those skilled in the art can make various changes or modifications to the present invention in light of the above teachings, and the equivalents also fall into the scope as defined by the appended claims of this application.

Claim 1:
A method for quantitatively co-expressing multiple proteins in vitro, comprising the steps of:
(<NUM>) establishing a standard curve:
establishing standard curve of protein concentration-luminescence intensity relationship for each co-expressed protein using corresponding standard protein;
(<NUM>) creating separate vectors containing each target protein gene for expressing each target protein respectively;
(<NUM>) establishing an equation of quantitative relationship between concentration percentage of each of target proteins and concentration percentage of the corresponding vector;
wherein the separate vectors in Step (<NUM>) containing the target protein genes are added at different concentration ratios to in vitro cell-free protein synthesis system for protein synthesis reaction; after a specified reaction time, a luminescence value for each target protein in the reaction solution is obtained; concentration of each target protein product is calculated according to the standard curve shown in Step (<NUM>), and an equation of quantitative relationship between concentration percentage of each target protein product and concentration percentage of the corresponding vector is obtained by fitting; in in vitro cell-free protein synthesis system, the total concentration of the vectors remains the same;
(<NUM>) calculating concentration and concentration ratio of the vectors for quantitatively co-expressing multiple proteins;
wherein, according to target concentration ratio relationship of the multiple target proteins to be expressed, the concentration and concentration ratio of the vector for each of the multiple target proteins to be expressed are calculated by using the equation established in Step (<NUM>);
(<NUM>) quantitatively co-expressing the multiple proteins;
wherein, according to the required concentration or concentration ratio of each target protein vector obtained in Step (<NUM>), corresponding amount of the independent vector of each target protein is added to the in vitro cell-free protein synthesis system as described in Step (<NUM>), and after the specific period of time defined in Step (<NUM>), the co-expressed multiple target proteins are obtained;
wherein the multiple target proteins are each independently luminescent protein or fusion protein carrying a luminescent label.