NZ530229A - The production of soluble keratin derivatives - Google Patents
The production of soluble keratin derivativesInfo
- Publication number
- NZ530229A NZ530229A NZ530229A NZ53022902A NZ530229A NZ 530229 A NZ530229 A NZ 530229A NZ 530229 A NZ530229 A NZ 530229A NZ 53022902 A NZ53022902 A NZ 53022902A NZ 530229 A NZ530229 A NZ 530229A
- Authority
- NZ
- New Zealand
- Prior art keywords
- keratin
- recited
- solution
- protein
- sulfonated
- Prior art date
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Abstract
Disclosed is a process for the preparation of keratin derivatives of high molecular weight, the process comprising a first stage digestion step of sulfonating a keratin source by oxidation sulfitolysis followed by a second stage repetitive aqueous extraction involving separation of soluble and insoluble keratin and subsequent re-extraction of the insoluble keratin to thereby produce a highly S-sulfonated keratin derivative.
Description
53022
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The Production of Soluble Keratin Derivatives Field of the Invention
This invention relates to a process for the preparation of derivatives of keratin 5 from animal sources such as wool, hair, horns, hooves, feathers and scales by an economic and environmentally acceptable process, and to a series of keratin derivative products produced thereby. Some of the keratin derivatives are soluble and can be used in the production of a range of biopolymer materials.
Background to the Invention
Keratins are a class of structural proteins widely represented in biological structures, especially in epithelial tissues of higher vertebrates. Keratins may be divided into two major classes, the soft keratins (occurring in skin and a few other tissues) and the hard keratins, forming the material of nails, claws, hair, horn, 15 feathers and scales.
The toughness and insolubility of hard keratins, which allow them to perform a fundamental structural role in many biological systems, are also desirable characteristics in many of the industrial and consumer materials currently derived 20 from synthetic polymers. In addition to possessing excellent physical properties, keratin, as a protein, is a material with a high degree of chemical functionality and, consequently, exhibits many properties that synthetic materials cannot achieve. Keratin is, therefore, well suited to the development of products with high-value, niche-market applications. Keratin is also an environmentally acceptable polymer 25 produced from a sustainable resource and therefore has environmental benefits
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over synthetic materials. Following the global trend of developing materials from renewable sources produced in a sustainable process, a range of materials has been produced from keratin, most commonly in the form of keratin films.
At the core of a new industry producing biopolymer materials from keratin it is essential to have a process for extracting keratin from its source that is economically viable, sustainable from an environmental perspective, and produces a stable and versatile product. Methods used to date for the extraction of keratin that maintain the integrity of the individual proteins have been designed for the 10 purpose of protein analysis and characterisation and consequently are not viable on an industrial scale, from an economic and environmental viewpoint. Methods used to date for the economic dissolution of keratin have significantly degrading effects on the protein, and consequently the dissolved protein retains few of the physicochemical properties that lead to the desirability of keratin as a biopolymer, 15 such as the ability to reconstitute into tough materials.
It' is an object of the invention to go some way in overcoming the disadvantages with known processes or at least provide the public with a useful choice.
In at least one embodiment the invention strives to provide an economic and environmentally acceptable process for the dissolution of keratin proteins that maintains the structural integrity and chemical functionality of the proteins during the dissolution process and leads to a stable and versatile keratin derivative product for the development of biopolymer materials.
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Summary of the Invention
According to a first aspect the invention provides a dissolution process for producing a range of stable, soluble keratin derivatives of high molecular weight, the molecular weight being similar to or greater than that of proteins originally 5 expressed in the keratin source, with little or no damage to the structural integrity of the constituent proteins. The dissolution occurs in a two-stage process.
According to a preferred aspect the invention provides a process for the preparation of keratin derivatives of high molecular weight, the process including a 10 first stage digestion step of S-sulfonating a keratin source by oxidative sulfitolysis followed by a second stage extraction step using controlled washing with water to thereby obtain a highly S-sulfonated keratin derivative.
The conversion of highly S-sulfonated keratin from a solid state into solution is 15 without the use of chaotropic agents, by controlled, gradual washing of the sulfonated keratin with water in order to wash out the residual chemical reagents from the extraction procedure and alter the ionic strength of the extraction solution.
The first stage involves oxidative sulfitolysis to convert cystine groups present in the protein to S-sulfocysteine, using industrially acceptable concentrations of inexpensive reagents for the purpose of sulfonation (eg. sodium sulfite) and oxidation (eg. cupraammonium hydroxide).
According to another aspect, the invention provides a process for the separation of a gelatinous keratin product from a solution of S-sulfonated keratin produced by
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the above process, wherein the S-sulfonated keratin derivative solution is treated by the use of a gentle, gravity fed filtration system followed by separation. Preferably the separation is centrifugal.
According to another aspect of the invention, a liquid stream remaining after the gelatinous keratin is removed is processed by passing over scoured wool, thereby removing residual chemicals from the solution and preparing the wool for subsequent protein extraction processes.
Following conversion of the cystine groups, the second stage of the process is one in which the highly S-sulfonted keratin derivative is brought from a solid or gelatinous state into solution by extensive dilution with water. The rate and extent of dissolution can be controlled by the use of heat, surfactants, gentle agitation and vigorous chopping or homogenisation. By controlling the rate of 15 dissolution, reaction solutions can be isolated, for example if a copper oxidant is used a reaction solution rich in copper is produced but it contains little or no dissolved protein, or are rich in protein but contain little or no copper.
According to another aspect of the invention, a liquid stream resulting from the 20 second stage of the process, which contains residual chemicals such as copper sulfate and sulfite, as well as S-sulfonated keratin derivatives, is processed using any one or more of a variety of methods that allow the recycling of reagents from the solution and the separate isolation of purified S-sulfonated Keratin Intermediate Filament Protein(s) (SIFP) and S-sulfonated Keratin High Sulfur Protein(s) (SHSP). 25 This is achieved through the use of chelating agents, such as ethylenediamine
PCT /N Z02/00125
tetraacetic acid, or chelating ion exchange resins, such as those containing the iminodiacetic functional group, and the use of isoelectric precipitation to separate protein types. Ultrafiltration can be used at several stages in the process to improve the efficiency of reagent removal or protein separation. Metallic impurities 5 in the protein products can be further reduced by the washing of the protein derivative(s) following precipitation with dilute acids, water or chelating agents. Once separated, the protein products can be dried by a range of methods such as fluid bed, spray or freeze drying.
Another aspect of the invention is the further processing of residual keratin not dissolved by the two stage sulfitolysis process, through the use of other reagents, such as hydrogen peroxide, sodium sulfide or proteolytic enzymes, to produce keratin peptides.
Another aspect of the invention is the provision of a method for large scale recovery of proteins from a natural source, including subjecting said natural protein source to a treatment sufficient to render at least some of the protein(s) water soluble, and subsequently separating the water soluble protein(s).
Another aspect of the invention is the provision of an installation for large scale recovery of proteins from a natural source, a treatment vessel to contain and subject a large quantity of natural protein source to a treatment sufficient to render at least some of the protein(s) contained in said feed, water soluble, and a 25 separation apparatus to subsequently separate the water soluble protein(s).
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Another aspect of the invention is a method of selectively solubilising a protein having plurality of disulfide bonds from a mixture of proteins including subjecting said mixture of proteins to oxidative sulfitolysis to produce a soluble S-sulfonated 5 protein fraction. The oxidative sulfitolysis is preferably effected in the absence of chaotropic agents with little or no damage to the structural integrity of the protein.
Another aspect of the invention is method for obtaining a purified protein from an 10 impure protein source with little or no damage to the structural integrity of the protein including subjecting said protein source to a treatment sufficient to render at least some of the protein(s) water soluble, and subsequently separating the water soluble protein(s) in the absence of chaotropic agents.
Description of Preferred Examples of the Invention
The combination of aspects that make up the process as a whole are summarized 20 diagrammatically in attached Figure 1.
This process method is for the preparation of highly sulfonated keratin derivatives and can be applied to any keratin source, such as animal wool, hair, horns, hooves, feathers or scales. Whilst the application of the method to different 25 keratin sources can give soluble keratins with different structure and properties, the fundamental step of the dissolution process, in which cystine is converted to s-sulfocysteine, applies equally well to all keratin-containing materials.
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The process can be conceived as occurring in two stages.
Stage one, which involves the conversion of cystine to S-sulfocysteine, occurs through a procedure of oxidative sulfitolysis. This can be achieved by the use of a 5 sulfonating agent, such as sodium sulfite or sodium metabisulfite, which asymmetrically cleaves the cystine to cysteine and S-sulfocysteine, and an oxidant, which converts the cysteine produced in sulfonation to cystine. By further sulfonation of cystine complete conversion of all cystine to S-sulfocysteine is achieved.
Oxidants which can be used include sodium tetrathionate, iodosobenzoate and cuprammonium hydroxide. In a preferred embodiment of this invention the sulfonating reagent used is sodium sulfite in the concentration range 0.02M to 0.2M and the oxidant used is cuprammonium hydroxide in the concentration range 15 0.02M to 0.08M, generated by the combination of copper sulfate and ammonia. The first stage of the procedure for solublising keratin is the soaking, for a residence time such as 24 hours, of the keratin source in a solution or sequence of solutions that convert the cystine to S-sulfocysteine, with a liquor to wool ratio (volume:weight) in the range 5:1 to 50:1.
In another embodiment of the invention the sulfonating agent used is sodium metabisulfite in the concentration range 0.1M to 0.5M, maintained at acidic pH. In this embodiment the wool is removed from the solution containing sodium metabisulfite before being added to a solution containing a cuprammonium 25 complex in the concentration range 0.02M to 0.08M.
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Previous work relating to the use of the oxidative sulfitolysis procedure has required the use of large concentrations of chaotropic agents, such as urea or guanidinium hydrochloride, in order to swell the keratin source and facilitate the dissolution of keratin. This procedure is both expensive and impractical on an industrial scale. Previous work relating to the use of oxidative sulfitolysis using copper as the oxidant has been conducted under conditions of temperature and pH that are detrimental to the integrity of the protein causing high rates of conversion of cystine to lanthionine.
Stage two of the process involves the conversion of highly sulfonated keratin from a solid state into solution without the use of chaotropic agents and under conditions of temperature and pH that maintain the structural integrity of the protein, by controlled, gradual washing of the sulfonated keratin with water in order to wash out the residual chemical reagents from the extraction procedure and alter the ionic strength of the extraction solution. This combination of effects results in the conversion of the highly sulfonated keratin from the solid state into aqueous solution. In the preferred procedure the reaction volume is replaced every 12 to 48 hours, either in a batch process or on a continuous basis.
The rate and extent of dissolution can be controlled by the use of surfactants, the action of heat, agitation, and homogenisation of the sulfonated keratin. A feature of the invention is to use these factors to control the rate of extraction. The highly S-sulfonated keratin can, therefore, be kept in the solid state and separated from the extraction solution containing the bulk of the chemicals used for the
PCT/N Z02/00125
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sulfonation process. The preferred procedure uses a non-ionic surfactant, such as Triton X 100 in the range 0.1% to 5% by weight, and a temperature maintained in the range 1 5°C to 50°C.
An advantage of the invention when a copper based oxidant is used is the re-use of this copper-rich extraction solution for subsequent extraction processes, significantly reducing both the cost and environmental impact of the process. Reuse of the copper-rich solution is possible due, in part, to the regeneration of the active copper species through aerial oxidation. One method in which the copper-10 rich solution can be efficiently reused is by passing the solution over wool. Wool binds copper from the solution, and if this wool is then used for subsequent extraction processes, the demand for copper in those subsequent extractions is reduced. In this way, a 'wool filter' can be used as a key step in the processing of the copper-rich extraction solution, reducing the subsequent need for effluent 15 treatment and also the need for copper to be added to the subsequent processes. In a typical procedure the liquid stream from stage 1 contained approximately 1800 - 1500 (parts per million) ppm copper, and after passing over the wool filter this was reduced to approximately 400 - 300ppm.
The first stage of the process, and the recovery of reagents for use in the process are indicated in the attached Figure 1.
After S-sulfonation and homogenisation the keratin material becomes a gelatinous swollen fibrous mass.
A further advantage of the invention is the separation of the highly S-sulfonated keratin derivatives in the solid state from solutions containing either chemicals used in the extraction process or the keratin protein in solution. This separation is effectively achieved by the use of a gentle, gravity based filtration through a fine 5 mesh screen, followed by centrifugal separation of the filtrate from fine particulates.
Solutions of highly S-sulfonated keratin derivatives can be purified with regard to metal ions, specifically the copper ions used as part of the extraction process, 10 through the use of ion exchange media, in particular those containing iminodiacetic acid functionality known to possess a high affinity for divalent metal ions. This ion exchange medium may be present in the form of a packed resin column, over which the protein solution is passed, or it may alternatively form part of an electrochemical cell, in which copper is recovered from the ion exchange medium 15 through the use of an applied voltage and a system containing permeable membranes.
Once the highly S-sulfonated keratin derivates are in solution particular proteins eg. the S-sulfonated keratin intermediate filament protein can be readily isolated by 20 isoelectric precipitation, around pH 4 or below, using acids such as sulfuric acid, hydrochloric acid, citric acid or acetic acid, with the preferred procedure using sulfuric acid. An advantage of the invention is the minimisation of the binding of copper and other metallic impurities to the protein prior to isoelectric precipitation through the use of ion exchange media as described, or by addition of a chelating 25 agent, such as ethylenediaminetetraacetic acid (EDTA), to the protein solution. In
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the preferred example EDTA (0.2M) is added to the liquid stream from stage 2 at a rate of 25ml per liter, or at a rate suitable to sequester all the copper ions present in solution as indicated by analysis of the solution. Metallic impurities can be further reduced by the washing of the protein, once isolated by precipitation, with 5 a dilute acid solution, or solution of a chelating agent such as EDTA, or water.
Following precipitation and washing the separated protein can be isolated in a stable, dry state using drying methods involving air flows at about ambient temperature, for example with the use of a fluid bed dryer. Alternatively, the
product can be dried using a freeze dryer. The dry protein product contains cystine groups in the form of S-sulfonic acid and consequently the protein is only soluble in the presence of a base, such as sodium hydroxide or ammonium hydroxide. These processes are represented as drying in the attached Figure 1.
The highly soluble keratin derivatives that remain in solution following isoelectric precipitation, which in the case of wool are mainly the high sulfur matrix proteins from within the wool fibre, can be isolated in a stable form from solution through a process of ultrafiltration, to remove non-proteinacious species such as residual copper or EDTA, followed by spray drying.
A feature of the invention is the use of a combination of isoelectric precipitation and ultrafiltration followed by spray drying to separate highly S-sulfonated keratins according to their properties in solution. In the case of wool keratin, this effectively separates the low sulfur intermediate filament protein class from the
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high sulfur matrix protein class and provides two product streams with different chemical properties.
A feature of the invention is the preparation of a stable, water soluble form of the 5 highly S-sulfonated keratin derivative, by dissolving the S-sulfonic acid form of keratin in the presence of base and spray drying the resulting solution.
A feature of the invention is the combination of engineering components to allow solublisation of the keratin and isolation of the S-sulfonated keratin from solution 10 in a continuous, semi-continuous, or batch process. This combination of engineering components and unit operations is detailed in Figure 1.
An advantage of the invention is the recovery and reuse of copper from the reaction mixtures and effluent streams of the process. Copper can be recovered 15 using electrochemical methods, including the use of selective permeable membranes in order to separate copper ions from EDTA prior to electrochemical deposition. Alternatively, immobilized binding agents, in the form of copper-specific ion exchange resins, can be used to remove copper from the effluent stream. Copper removed using these methods can be reused, thereby minimizing 20 the environmental impact of the process.
The use of ion exchange media and/or chelating agents is represented as purification in the attached Figure 1.
PCT/N Z02/00J 25
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Another advantage of the invention is the further processing of residual keratin which remains in the solid state following the extraction procedure. This functionalised keratin is highly S-sulfonated, therefore the disulfide bonds present in the native keratin that render it resistant to chemical and enzymatic attack have 5 been cleaved and the keratin is readily digestible using other extraction methods. For example, a solution rich in keratin peptides can be prepared through the action on this residual keratin of alkaline solutions of a strong oxidant such as hydrogen peroxide, in the concentration range 10-100ml of 50% hydrogen peroxide per kg of the keratin residue under alkaline conditions. The keratin residue contains 10 approximately 5% solids. Alternatively, solutions of strong reductants such as sodium sulphide in the concentration range 0.5%-15% added to the keratin residue can be used to prepare a solution rich in keratin peptides. Alternatively, proteolytic enzymes, such as those of the subtilisin, papain or trypsin groups, can be employed at levels in the range 0.1 mg - 20mg of enzyme per gram of keratin 15 residue at temperature and pH conditions appropriate for the specific enzyme to readily digest the residual keratin and prepare a solution rich in keratin peptides. All of these methods result in the formation of a solution rich in keratin peptides which can be processed in a similar manner to the liquid stream resulting from stage 2 described above, that is through the use of ion exchange media, pH 20 adjustment and drying (shown as purification and drying in Figure 1), to produce keratin peptide solids. Digestion of the keratin residue in this way minimises the keratin waste produced by the process as a whole, and ensures maximum utility of the keratin protein present in the keratin source.
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The two intact protein products from the process are S-sulfonated keratin intermediate filament protein and S-sulfonated keratin high sulfur protein. The S-sulfonated keratin intermediate filament protein typically produced by the process was analysed using sodium dodecylsulfate polyacrylamide gel electrophoresis 5 (SDS-PAGE) analysis using a reduction/alkylation procedure, which indicated a molecular weight distribution predominantly in the range 30-60kD (intermediate filament proteins), with a small component of protein of mass 10kD (high glycine high tyrosine proteins). The amino acid composition of this product is given in Table 1 and is typical for wool keratin intermediate filament proteins. The S-10 sulfonated keratin high sulfur protein was analysed using SDS-PAGE after a reduction/alkylation procedure, which indicated a molecular weight predominantly in the range 1 5-20kD. The amino acid composition of this product is given in Table 1 and is typical for wool keratin high sulfur proteins.
Cya
Asp
Glu
Ser
Gly
His
Ar9
Thr
Ala
Pro
Tyr
Val
Met
Lan lie
Leu
Phe
Lys
Cys
SIFP
0.4
7.9
.4
.9
8.1
0.9
7.9
6.5
7.5
.4
1.1
6.5
0.2
0.2
3.7
8.9
2.5
2.1
4.2
SHSP
1.7
2.6
8.6
14.3
9.1
0.8
6.8
.4
3.6
12.6
1.8
6.3
0.0
0.2
2.9
3.9
1.5
0.4
12.4
IFP
0.0
9.6
16.9
8.1
.2
0.6
7.9
4.8
7.7
3.3
2.7
6.4
0.6
0.0
3.8
.2
2.0
4.1
6.0
HSP
0.0
2.3
7.9
13.2
6.2
0.7
6.2
.2
2.9
12.6
2.1
.3
0.0
0.0
2.6
3.4
1.6
0.6
22.1
Table 1: amino acid composition of S-sulfonated keratin intermediate filament protein (SIFP). S-sulfonated keratin high sulfur protein (SHSP), intermediate filament protein (IFP) and high sulfur protein (HSP) (later two courtesy of Gillespie and Marshall, Variability in the proteins of wool and hair, Proc. Sixth Int. Wool Text. Res. Conf., Pretoria, 2, 67-77, 1980). All residues expressed as mol%. S-sulfocysteine, cystine and 20 cysteine are measured as S-carboxymethyl cysteine following reduction and allcylation.
An example of the process is shown diagrammatically in the attached Figure 1. Ultrafiltration is considered as being a possible component in each purification stage. The key components are illustrated by the following examples of a protein 25 extraction procedure.
Examples:
Example 1 Stage 1, Digestion
The digestion stage of the process involves the use of oxidative sulfitolysis to convert cystine to S-sulfocysteine within the keratin source.
Example la. stage 1, digestion
In order to extract the keratin from 10kg of wool, firstly 2kg of copper sulfate pentahydrate was mixed using a high shear mixer with eight litres of concentrated ammonia. This mixture was diluted to 200L with water and 10kg of wool was added. Approximately 15L of sulfuric acid (2M) was added to the stirred mixture 10 till a pH 9.4 was achieved. Anhydrous sodium sulfite (5.04kg) was added and the solution mixed until complete dissolution of all of the reagents had occurred and the pH stabilised at 9.5. The final concentration of the cupric ammonia complex was 0.04M. The sodium sulfite had a final concentration of 0.2M. The temperature of the digestion solution was maintained at 20°C. After 24 hours of 15 gentle agitation the fibrous gelatinous mass of softened wool was filtered. The filtrate was passed through a fresh wool filter, which decreased the copper level in the solution from 1725ppm to 130ppm, and further purified using Purolite S930 IDA ion exchange resin, which under acidic conditions further reduced the copper level to 12ppm. Fresh water was added to the softened wool and the mixture was 20 agitated.
Example 1 b. stage 1, digestion with the use of surfactant.
In a variation of example 1a, the digestion solution was prepared with the addition of 1 % of a non-ionic surfactant Triton X 100. The addition of this surfactant resulted in a delay in the release of soluble protein from the fibre, allowing a more
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effective separation of protein from residual reagents such as copper salts in the extraction solution.
Example 1c. stage 1, digestion.
In a variation of example 1a, the digestion stage occurs in two parts. In the first 5 part wool is pretreated with sodium metabisulfite at a concentration of 0.2M, at pH 4.2. Following removal of the wool from this solution, and with no attempt to remove residual sulfite from the wool, the wool was immersed in a cuprammonium hydroxide solution, at the concentration and pH described in example 1a for a further 24 hours at 20°C.
Example 2. Stage 2, Extraction.
Example 2a. stage 2, batch extraction.
Following completion of stage 1, described in examples 1, the mixture was agitated for a period of 16 hours, before being homogenized. Following a further 4 hours of agitation the solids and solution were separated using a two-stage 15 filtration process involving a wedge wire screen followed by a settling tank and a spinning disc centrifuge. The solid phases were returned to the reaction vessel and water was added to give a final liquor to wool ratio of 20:1 based on original wool solids. Following 24 hours agitation or continuous homogenisation the mixture was separated by repeating the two-stage filtration process. The solid 20 phases were returned to the extraction vessel and further diluted. This cycle was repeated 7 to 12 times. The liquid phases, containing soluble proteins, were further processed as detailed below in example 3.
Example 2b. stage 2, continuous extraction.
Following completion of stage 1 the mixture was processed as described in 25 example 2a, except that the two stage filtration process occurred on a continuous
WO 03/011894 PCT/NZ02/00125
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process, and solids and fresh water were added to the reaction tank at a rate equivalent to the volume of the tank being replaced in 24 hours. This process, was continued for 120 hours.
Example 3. Processing of protein solutions.
Ultrafiltration can be used at several points during the processing of protein solutions, in order to concentrate solutions and make the processes of drying and ion exchange more efficient. Ultrafiltration may be used prior to any processing step outlined in the following examples.
Example 3a. processing of protein solutions using EDTA 10 The solution produced as a result of stage 2, as described in Example 2, was further processed to isolate purified soluble keratins. EDTA (0.2M ) was added to the liquid phase at a rate of 25mL per liter, or at a rate suitable to sequester all the copper ions present in solution as indicated by analysis of the solution. Following 1 hour of mixing, the pH of the filtrate was reduced to 3.5 using sulfuric acid.
The protein precipitate was isolated using a screen, and washed sequentially with dilute sulfuric acid and water. The protein, S-sulfonated keratin intermediate filament protein, was dried by one of three routes, freeze drying, fluid bed drying or spray drying following dissolution with dilute sodium hydroxide. The filtrate 20 following the protein precipitation procedure was further processed using ultrafitration, to separate the protein components from the residual reagents. The retentate was spray dried to isolate further soluble protein, S-sulfonated keratin high sulfur protein. The permeate was further processed to recover copper and EDTA from the effluent stream using ion exchange media.
Example 3b. processing of protein solution using ion exchange media
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The solution produced as a result of stage 2, as described in Example 2, was further processed to isolate purified soluble keratins. The liquid phase was passed over ion exchange resin, such as the chelating resin Purolite S930 IDA ion exchange resin containing the iminodiacetic acid functional group, in order to remove copper ions from the solution. Following ion exchange the pH of the filtrate was reduced to 3.5 using sulfuric acid and further processed in an identical manner to that described for Example 3a.
3c. processing of protein solution using pH adjustment prior to ion exchange.
The solution produced as a result of stage 2, as described in example 2, was further processed to isolate purified soluble keratins. The pH of the liquid phase was reduced to 3.5 using sulfuric acid. The protein precipitate was isolated using a screen, redissolved using dilute sodium hydroxide and further purified with either the addition of EDTA or by passing over an ion exchange column. Following further purification, the pH of the solution was reduced to 3.5 using sulfuric acid and the protein was isolated as described in the earlier examples. The filtrate from the initial pH reduction step, which still contains significant amounts of soluble protein and other reagents, was purified by passing over ion exchange media and spray dried to isolate further soluble protein, S-sulfonated keratin high sulfur protein.
Example 4. Dissolution of residues from stage 2
The solid stream isolated as a result of stage 2 can be further processed to produce keratin peptides by a range of methods. The high level of sulfonation of the residue makes it readily amenable to chemical and enzymatic digestion, as the disulfide bonds present in the original keratin source resistive to chemical and enzymatic attack have largely been cleaved.
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Example 4a dissolution of residues using sodium sulfide
Sodium sulfide solution (5% by weight) is added to an equal volume of the solid stream from stage 2 of the process, which comprises approximately 5 % solids. The mixture is agitated for 1 2 hours after which time the solids are removed by 5 filtering and centrifugation and sulfuric acid is added to the protein solution to decrease the pH to the range 2 to 3.5. The precipitate is collected on a screen and washed thoroughly with water.
Example 4b dissolution of residues using hydrogen peroxide
Hydrogen peroxide (50%) is added to the solid stream from stage 2 at a level of 10 25-30 ml per kg of keratin residue (keratin residue contains approximately 5% solids). This is mixed and 1M sodium hydroxide is added to obtain pH in the range of 10 to 13. The mixture is agitated gently for 24 hours and the protein and solids separated by the two stage filtration process described in Example 2 and protein isolated by acidification as described in Example 4a. Alternatively the protein 15 solution is passed over an ion exchange resin, then acidified and the precipitated solid collected. The acidified solution may then be passed through an ion exchange column prior to freeze-drying or spray drying to collect a further protein-rich product.
4c dissolution of residues using proteolytic enzymes
An industrial subtilisin enzyme preparation (a solution containing 2.5% active enzyme) was added to the solid stream from stage 2 in the amount of 10mg of active enzyme per gram of keratin residue. The pH was maintained at 9.5 with the addition of sodium hydroxide and the reaction heated to 60 °C for 2 hours. The resulting protein solution is isolated from solids and processed as described in 4a
or passed through ion-exchange resin prior to and/or following acidification as described in 4b.
Thus by the invention there is provided a method for the production of soluble keratin derivatives that is both economic and environmentally acceptable.
Particular examples of the invention have been described and it is envisaged that improvements and modifications can take place without departing from the scope of the attached claims.
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Claims (26)
1. A process for the preparation of keratin derivatives of high molecular weight, the process including a first stage digestion step of sulfonating a keratin source by oxidative sulfitolysis followed by a second stage repetitive aqueous 5 extraction involving separation of soluble and insoluble keratin and subsequent re-extraction of the insoluble keratin to thereby produce a highly S-sulfonated keratin derivative.
2. A process according to claim 1 wherein the first stage is carried out without the use of a chaotropic agent. 10
3. A process according to claim 1 or claim 2 wherein the first stage is carried out under conditions of pH that maintains structural integrity of the protein.
4. A process as recited in any preceding claim in which the oxidative sulfitolysis uses cuprammonium hydroxide, or a thionate, as the oxidant, and sulfite.
5. A process as recited in any preceding claim wherein the two stages use 15 surfactants, heat, agitation and homogenisation to control the rate of digestion in the first stage and extraction in the second stage.
6. A process as recited in claim 4 using surfactants, heat, agitation and homogenisation to control the rate of release of residual reagents and soluble protein, thereby allowing separation of the highly S-sulfonated keratin 20 derivative.
7. A process for the separation of a gelatinous keratin substrate from the solution of S-sulfonated keratin produced by the process as recited in any one of claims 1 to 6 wherein the S-sulfonated keratin derivative solution is treated by the use of a gravity fed filtration system followed by centrifugal separation. 25
8. A process as recited in claim 1 wherein the solution of S-sulfonated keratin is purified using chelating agents, such as EDTA, to sequester metal ions, such as copper.
9. A process as recited in claim 1 wherein the solution containing S-sulfonated keratin derivatives is purified using ion exchange media to remove residual 30 reagents, including metals such as copper. IPONZ 2 3 AUG 2006 22
10. A process as recited in claim 9 wherein the solution is concentrated prior to an ion exchange treatment through the use of ultrafiltration membranes, or similar. 5
11. A process as recited in claim 10 in which reagents such as copper are isolated and reused in subsequent processes.
12. A highly S-sulfonated solution of keratin derivatives produced by the process of any one of claims 1 to 11.
13. A process for the isolation of highly S-sulfonated keratin intermediate filament 10 proteins from the solution of keratin claimed in claim 12 wherein the highly S- sulfonated keratin intermediate filament protein is isolated by isoelectric precipitation at acidic pH.
14. A highly purified proteinaceous product produced by the process of claim 13.
15. A proteinaceous product as recited in claim 14 which is purified by the 15 dissolution of the S-sulfonated keratin intermediate filament proteins in base in the presence of EDTA, and subsequently precipitated at acidic pH.
16. A water soluble form of S-sulfonated keratin intermediate filament protein produced by spray drying an aqueous solution of the polymeric product as recited in claim 14. 20
17. A process for the production of highly S-sulfonated keratin high sulphur proteins, produced by spray drying the solution of S-sulfonated keratin derivatives purified as claimed in claims 8 or 9, and after having had the intermediate filament proteins removed by the process as claimed in claim 13.
18. A proteinaceous product produced by the process of claim 17. 25
19. A process for the production of soluble keratin peptides through the action of hydrogen peroxide solutions on the gelatinous residue produced by the process as recited in any one of claims 1 to 7.
20. A proteinaceous product produced by the process recited in claim 19.
21. A process for the production of soluble keratin peptides through the action of 30 sodium sulfide solutions on the gelatinous residue produced by the process as recited in any one of claims 1 to 7.
22. A proteinaceous product produced by the process recited in claim 21. IPONZ 2 3 AUG 2006 23
23. A process for the production of soluble keratin peptides through the action of proteolytic enzymes, such as those from the subtilisin, papain or trypsin families, on the gelatinous residue produced by the process as recited in any 5 one of claims 1 to 7.
24. The proteinaceous product produced by the process recited in claim 23.
25. A process for the treatment of copper-rich solutions produced by the process as recited in claim 4, in which wool is used as a filter media to bind copper and remove it from the solution. io
26. A subsequent protein extraction process for the treatment of the copper-laden wool produced by the process recited in claim 25. IPONZ 23 AUG 2006
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| NZ530229A NZ530229A (en) | 2001-07-17 | 2002-07-17 | The production of soluble keratin derivatives |
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| NZ51272501 | 2001-07-17 | ||
| NZ530229A NZ530229A (en) | 2001-07-17 | 2002-07-17 | The production of soluble keratin derivatives |
| PCT/NZ2002/000125 WO2003011894A1 (en) | 2001-07-17 | 2002-07-17 | The production of soluble keratin derivatives |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| NZ530229A true NZ530229A (en) | 2006-11-30 |
Family
ID=37500066
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| NZ530229A NZ530229A (en) | 2001-07-17 | 2002-07-17 | The production of soluble keratin derivatives |
Country Status (1)
| Country | Link |
|---|---|
| NZ (1) | NZ530229A (en) |
-
2002
- 2002-07-17 NZ NZ530229A patent/NZ530229A/en not_active IP Right Cessation
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