Abstract:
Lysozyme from human, avian, non-human mammalian, and vegatable sources is isolated from said sources and provided in a high degree of purity by adsorbing the lysozyme upon chitin obtained from Loligo vulgaris by contacting said chitin with an acidic aqueous suspension of the crude lysozyme containing material, and eluting the pure lysozyme from said chitin with aqueous acid.

Description:
FIELD OF THE INVENTION 
     Isolation of pure lysozyme. 
     BACKGROUND OF THE INVENTION 
     Lysozyme is a highly active enzyme which was originally isolated by Fleming during his early work on penicillin. Lysozyme is found in mammalian, including human, tissues and body fluids such as blood, tears, and milk as well as in avian sources, such as avian egg-white and vegetable sources. It is also found in bacteria and bacteriophages. The major sources of lysozyme to date has been avian eggs and various methods are known for the isolation thereof in reasonable degrees of purity. These procedures however are lengthy, tedious, and expensive and do not lend themselves readily to production scale isolation of lysozyme. Lysozyme from avian sources may be used as a food preservative. It has long been considered a highly desirable preservative since it may be passed into the human digestive system with no adverse effects thereto and does not suffer from the problem of chemical residue which effects many artificial preservatives. Unfortunately however the cost factor heretofore involved in producing large amounts of pure lysozyme have, in effect, prevented its large scale utilization for this highly desirable purpose. 
     Since lysozyme operates as a bacteriolytic agent it is of potential use as a potentiator for drugs such as antibiotics and the like. Unfortunately, heretofore there have been certain immunological barriers to its use for this purpose. While avian and non-human lysozyme may be ingested by humans without adverse immunological effects non-human lysozyme will set up antibody reactions when ininjected into the human circulatory system. When lysozyme from human sources is injected into the human circulatory system antibody response is sometimes obtained and sometimes not obtained. The only way of ensuring absolutely that no antibody response would be obtained would be to inject lysozyme obtained from the injected subject itself together with the desired drug. Thus, it would be desirable to develop a method for efficiently separating lysozyme from a human subject in such a way that the supplying constituents of that subject are not otherwise degraded. Similarly, since there are known tests for antibody response, if human lysozyme can be readily obtained from other human sources, it is a comparatively simple job of testing to determine whether or not a subject would exhibit antibody response if foreign human lysozyme were injected into that human system. 
     Heretofore the available methods of isolating lysozyme from human sources have not been sufficiently efficient either to supply an adequate amount of lysozyme in sufficient purity to ensure that no antibody response due to other protein sources would be invoked, or, the methods available for the supply of pure lysozyme have been so expensive as to be worthless from a practical, that is to say, nonacademic point of view. 
     Chitin is a known material which may be obtained from various marine sources such as crabs and the like. Chitin from crabs has been utilized in procedures for the isolation, but not purification, of lysozyme. 
     SUMMARY OF THE INVENTION 
     It has been found that chitin isolated from the squid (Loligo vulgaris) after being subjected to deamination provides an absorptive medium which specifically removes lysozyme from aqueous, slightly acid, suspensions containing same. The lysozyme may then be readily removed from the chitin by washing with aqueous dilute acid from which the lysozyme itself may be isolated by methods well known to the art. It is a specific advantage of this reaction that in one isolation step the concentration of lysozyme may be raised from about 1500 to 10,000 times. 
     It is a further advantage of this method that it is operative regardless of the source of lysozyme, that is to say, mammalian (human or non-human, avian or vegetable). 
     The lysozyme which is isolated by means of the preferred embodiments of the present invention is of high purity. 
     DESCRIPTION OF THE PREFERRED EMBODIMENTS 
     The process of the present invention can be conveniently divided into two parts. The first being the preparation of the absorption material and the second being the absorption procedure itself. 
     The chemical substance, chitin, which is utilized as the adsorbant material is found in many forms of marine life, such as the skeleton of arthropods, annelids, molusks medusoid coellenterates, in nematodes and achantocephalans. Only chitin isolated from the pens of the squid (Loligo vulgaris) was found suitable for use as a selective absorbant for lysozyme. While we do not wish to be bound by any theory, it is believed that this desirable property is due to the anti-parallel orientation of the chains of chitin in the physical form in which they are found. By anti-parallel is meant that the structural units are oriented parallel to each other but the directional sequence of the atoms in each structural unit alternates from one chain to the adjacent chain thereto. 
     The squid pens are removed from the animal and washed free of flesh, suitably with running tap water. The material is then dried overnight at moderately elevated temperature. Temperatures above 70°C but below 100°C, being suitable, 95°C being particularly desirable. The material is then cut into small pieces, suitably having dimensions in any direction of 1 centimeter or less and saline is added thereto. The purpose of the saline is to provide a suitable homogenization medium. The amount and concentration of saline is not critical, however, it has been found suitable to utilize from about 5 to about 20 suitably about 10 volumes of 0.1 to 5 normal, suitably about 1 normal aqueous sodium chloride. The mixture is then homogenized in a suitable rotating blade grinder at the highest speed available thereto. Homogenization is continued for from about 30 minutes to about 2 hours, suitably for about one hour, the mixture is removed from the homogenization unit, the supernatant liquid removed and discarded and made up once more to the original volume with more saline. It has been found desirable to sharpen the blades of the mixture between each homogenization step. This procedure is repeated from one to about five times, suitably 3 times. After discarding the last supernate, it is desirable to remove any residual fatty material. While any dilute water soluble acid may be utilized in this step, it has been found especially suitable to utilize water soluble organic acids and particular acetic acid in a strength of from about 0.5 to 2 suitably about 1 molar. The residual chitin is re-suspended in about 10 volumes of acid and homogenized once more for about one hour in the same or similar equipment. After homogenization the supernate is again discarded and the residual chitin is first dried, suitably at above 70°C but below 100°C preferably at about 95°C for a few hours, suitably overnight and pulverized, suitably in a ball mill to a powder of between 100 and 400 mesh. While any mesh in this range is suitable it has been found that chitin of approximately 100 mesh possesses the most desirable combination of available surface area, coupled with particulate size great enough to permit a good flow therethrough when used in a chromatographic column. 
     The chitin is then deaminated by any deamination method known to the art, it has been found particularly suitable to carry out the deamination by the Van Slyke procedure. The chitin is treated with nitrous acid to convert the amino groups thereon into hydroxy groups to yield desaminopolyhydroxy squid chitin. Any convenient source of nitrous acid may be employed, in the preferred procedure  one part of chitin, 3 parts of glacial acetic acid and 9 parts of 30% aqueous sodium nitrite are agitated for about 24 hours. The thus treated material is then washed. In the preferred washing procedure the deaminated chitin is placed on a sintered glass filter, and washed with distilled water and suction until the effluent pH is above pH 5.5. 
     While any means of contacting the source of lysozyme with the squid chitin may be employed, it has been found must efficient to pack the chitin into a chromatographic column. It is preferred to prepare such chromatographic columns by gravity flow followed, preferably by washing with acetic acid, suitably with about 100 column volumes of acetic acid followed by distilled water until the pH of the effluent is again above pH 5.5. 
     PREPARATION OF LYSOZYME SOURCES FOR LYSOZYME EXTRACTION 
     While the preferred method of extracting lysozyme from its source is by chromatography through a chitin column it will be recognized that due to the diversity of the lysozyme sources somewhat different methods of pre-preparation have to be employed. It will be recognized that lysozyme constitutes a very small proportion of its source material which comprises to a greater or lesser extent, fibrous, particulate, or fatty materials. It will be understood that these and similar materials which constitute the major portion of the materials which contain lysozyme would seriously interfere with chromatographic extraction of lysozyme and must therefore be removed. 
     The basic principle in the following purification steps is the finding that the maximum aqueous solubility of lysozyme occurs between pH 3.8 and 4.6 and a pH of 4.5 is the most preferred. The methods of separation will of course depend on the nature of the source of material. 
     Where the source material is tissue material among which may be listed lung tissues, skin tissues, and, most suitable to all, placenta, tissues are cut into small pieces and homogenized in acidic solution preferably in a water soluble organic acid, most preferably .001M acetic acid in a conventional blender at high speed until complete disruption of the cells, followed by stirring in the cold (between about 0°C and about 5°C) for from about 5 to about 20, suitably from about 10 to about 21 days. 
     In the case of body fluids such as serum, plasma, saliva, or tears homogenization is not necessary. These fluids are diluted one-to-one with aqueous acid as above, suitably with 0.001M acetic acid, and is similarly stirred in the cold for from about 5 to about 20 days, suitably for about 10 days. Certain body fluids such as milk and colostrum have a high lipid content which must be removed. In these cases, the fluid is acidified to pH 4.5, suitably with 0.01M acetic acid and centrifuged. Three layers are noted, a top lipid layer, a central aqueous layer and a residue comprising denatured proteins and casein. Only the middle aqueous layer is utilized. Where the source of lysozyme is vegetables such as onions, radishes, papaya, and the like, these are processed in the same manner as tissues. Sources such as bacteriophage and certain bacteria, such as Staphylococcus aureus, Streptococcus viridans and Streptococcus faecalis which contain cellular material, are treated in the same manner as tissues. 
     Avian sources such as the egg-whites of hens, ducks, turkey, and fowls, are diluted 1:3 or 1:4 with 0.01M acetic acid with moderate stirring, the pH adjusted if necessary to pH 4.5, stood overnight at cold and centrifuged at high speed for the removal of particulate matter. 
     The aqueous acidic layers from each of the above sources contain the lysozyme dissolved therein but also contain fine particulate or pseudo-colloidal material which may very rapidly inactivate the chitin adsorbant. These aqueous layers are then centrifuged. Centrifugation may be for from about 1 hour at 8,000 g. to about 3 hours at 50,000 g. It has been found however that entirely satisfactory results are obtained by centrifugation for 2 hours at 30,000 g. 
     The aqueous supernate from this centrifugation is then contacted with the squid chitin. 
     ISOLATION OF LYSOZYME 
     While any mode of contacting the chitin with the lysozyme solution followed by removal of the lysozyme from the chitin may be used, the simplest and most effective mode is column chromatography wherein the aqueous acetic solution of the lysozyme is passed through a column of squid chitin and the lysozyme eluted therefrom with a suitable eluent. 
     In the preferred mode of carrying out the chromatography the lysozyme containing solution is charged to the squid chitin column through a delivery vessel at a controlled rate of flow. The optimum flow rate will of course depend on a number of factors, principally the mesh size of the chitin. However, it has been found that utilizing a chitin size of 100 mesh a flow rate of between 10 and 50 suitably 15 to 25 ml./cm squared of column cross-sectional area/per hour gives rise to suitable results. After passage of the lysozyme containing solution through the column the column is thoroughly washed with distilled water. The amount of wash is not critical however between about 8 and about 15 suitably about 12 column volumes of distilled water have been found satisfactory. 
     The lysozyme is then eluted with aqueous acid. There may be utilized mineral acids or water soluble organic acids. For example, there may be utilized dilute aqueous hydrochloric acid suitably of 2N strength or dilute aqueous sulfuric acid of .001 normal strength. There may also be used water soluble organic acids which may either be alkyl, aryl, aralkyl or alkaryl carboxylic acid. Especially preferred however are substantially volatile water soluble organic acids such as lower alkanoic acids having between 1 and 5 carbon atoms. It has been found especially suitable to utilize 0.01M acetic acid since not only is lysozyme readily soluble in this acid at this strength but the acid itself is sufficiently volatile to be readily removed by evaporation or lyophilization. 
     While other acids are operative it has been found that the highest yields at the highest purity have been obtained utilizing acetic acid. It has been found that the lysozyme is eluted in about 7 column volumes, the major portion being eluted in the second to fourth column volumes. 
     The course of the elution being followed by UV absorption at 280nm. 
     The lysozyme activity of each fraction is assayed by a modification of the method of Shugar (1951, Bull.Soc. Chim.Biol.33, 710 ) by recording the rate of lysis of a suspension of heat killed Micrococcus lysodeikticus (Sigma) (0.030 mg./100 ml. in 0.1M sodium phosphate buffer pH 7.00). A decrease in absorbancy of 0.001 per minute is taken as a unit of lysozyme activity. 
     The amount of protein is estimated according to the method of Lowry, Rosebrough, Farr and Randall (1951, J.Biol.Chem., 193, 265). 
     In a properly conducted isolation, a test of lysozyme activity in the effluent or in the washing shows 0(zero) biological activity against the micrococcal suspension. With the application of the eluent, the lysozyme is eluted with a recovery greater than 99%. 
     The eluted lyzosyme is concentrated first by flash evaporation, or under reduced pressure. If the eluate is not yet homogeneous, it is heated for 1-2 minutes at 100°C on a water bath, centrifuged for 1-2 hours at high speed for the removal of the denatured material, and the supernate brought to dryness by flash evaporation under reduced pressure of lyophylization. 
     The purity of this product was tested by disc gel electrophoresis as well as isoelectric focusing. These tests all showed a single band of protein moving with the same velocity as purified hen egg-white lysozyme which has been used as a control. 
     Immunological analysis was carried out upon the purified lysozyme obtained from different human tissues from different subjects by injecting the lysozyme into different rabbits and assaying the antibodies thus generated. The results obtained indicate prima facie that immunologically, though not necessarily chemically, all the human lysozymes tested appear to be identical. 
     The results obtained in the isolation of lysozymes from different sources by the method of the present invention are summarized in the tables below. 
    
    
     EXAMPLE I 
     CHITIN STRUCTURAL UNIT ##SPC1## 
     HUMAN LUNG LYSOZYME 
     Isolation by affinity chromatography on deaminated chitin. 
     column: diameter 12 mm; height 295 mm; bed volume 33.3 ml; grain 200-400 mesh. 
     Adsorption washings and elution at constant flow rate 20 cc/hour. 
     Washed with distilled water pH 6.5; Eluted with 0.01M acetic acid. 
     
         __________________________________________________________________________                    Specific                          Purification        Lysozyme             Proteins                    Activity                          Sp.Act/Sp.ActFraction   ml   Units             ng.    Units/ng                          in homogenate__________________________________________________________________________Lunghomogenate   100  3,700             3,250,000                    0.001138                          1Filtrate   100  0    3,180,000Wash    1,050        0    66,050Recovery in LysozymeInactiveFractions   1,150        0    3,246,050 %           0    99.89Eluate No. 1   10   200  160    1.250000                          1,0982       10   370  300    1.233333                          1,0843       10   540  430    1.255814                          1,1064       10   690  550    1.254545                          1,1025       10   840  680    1.235529                          1,0866       10   610  480    1.270833                          1,1177       10   320  250    1.280000                          1,1258       10   120  120    1.200000                          1,054Recovery in LysozymeActiveFractions   80   3,690             2,960 %           99.73             0.0009AVERAGE ENRICHMENT IN LYSOZYME × 1,097__________________________________________________________________________ 
    
     EXAMPLE II 
     HUMAN SKIN LYSOZYME 
     Isolation by affinity chromatography on deaminated chitin. 
     column: diameter 12 mm; bed height 425 mm.; bed volume 48.0 ml. DeCh grain size: 200-400 mesh 
     Adsorption, washing and elution at constant flow of 16 cc/hour. 
     Washing with distilled water (pH 6.4). Eluant 0.001 M AcOH 
     
         __________________________________________________________________________                       Specific                             Purification           Lysozyme                Proteins                       Activity                             Sp.Act/Sp.ActFraction   ml      Units                ng     Unit/ng                             in homogenate__________________________________________________________________________Skinhomogenate   400     2,000                12,800,000                       0.000156                             1Filtrate   400     0    12,400,000Wash    1,020   0    350,020Eluate No. 1   12.5    375  275    1.363636                             8,7412       12.5    750  538    1.395349                             8,943       12.5    500  375    1.333333                             8,9474       12.5    250  188    1.333333                             8,5475       12.5    125  125    1.428571                             9,158Recovery:In Lysozyme   inactive   fractions         0    12,750,020              (99.61%)In Lysozyme   active   fractions         2,000              1,501         (100%)              (0.0001%)AVERAGE ENRICHMENT IN LYSOZYME × 8788__________________________________________________________________________ 
    
     EXAMPLE III 
     HUMAN PLASMA LYSOZYME 
     Isolation by affinity chromatography on deaminated chitin. 
     column: diameter 12 mm; DeCh height 275 mm; bed volume 31.1 ml.; DeCh grain size: 200-400 mesh. 
     Adsorption, washings and elution at constant flow rate of 18 cc/hour. 
     Washings with distilled water, pH 6.6; elution with 0.01M AcOH 
     
         __________________________________________________________________________                    Specific                          Purification        Lysozyme             Proteins                    Activity                          Sp.Act/Sp.ActFraction   ml.  Units             ng     Units/ng                          in homogenate__________________________________________________________________________Plasmahomogenate   250  9,000             13,725,000                    0.000650                          1Filtrate   250  0    13,700,000Washings   1,260        0    12,600Eluate No. 1   15   1,650             1,500  1.500000                          2,3082       15   4,350             3,750  1.380950                          2,1253       15   2,100             1,400  1.400000                          2,1544       15   750  600    1.250000                          1,9235       15   150  110    1.363636                          2,098Recovery:In Lysozyme   inactive   fractions         O U   13,721,000 ng         (0%)  (99.91 %)In Lysozyme   active   fractions         9,000 U               6,860 ng         (100%)               (0.005%)AVERAGE ENRICHMENT IN LYSOZYME × 2,122__________________________________________________________________________ 
    
     EXAMPLE IV 
     HUMAN SERUM LYSOZYME 
     Isolation by affinity chromatography on deaminated chitin 
     column: diameter 10 mm; height 135 mm; bed volume 10.9 ml. grain size: 200- 400 mesh. 
     Adsorption, wash and elution at constant flow rate: 18 cc/hour. 
     Washed with distilled water (pH 6.5), eluted with 0.01M acetic acid. 
     
         __________________________________________________________________________                    Specific                          Purification        Lysozyme             Proteins                    Activity                          Sp.Act/Sp.ActFraction   ml.  Units             ng     Units/ng                          in homogenate__________________________________________________________________________Homogenate   100  1,200             5,732,000                    0.000209                          1Filtrate   100  0    5,620,000Wash    1,100        0    98,100Recovery in LysozymeInactivefractions   1,200        0    5,718,100 %           0    99.76Eluate No. 1   10   90   80     1.125000                          5,3722       10   300  240    1.250000                          5,9693       10   500  380    1.315779                          6,2964       10   260  220    1.181818                          5,6445       10   50   40     1.250000                          5,969Recovery in LysozymeActivefractions   50   1,200             960 %           100  0.02AVERAGE ENRICHMENT IN LYSOZYME × 5,850__________________________________________________________________________ 
    
     EXAMPLE V 
     HUMAN PLACENTA LYSOZYME 
     Isolation by affinity chromatography on deaminated chitin. 
     column: diameter 12 mm; height 435 mm; bed volume 49.2 ml. grain size: 200- 400 mesh. 
     Adsorption, washings and elution at constant flow: 20 cc/hour. 
     Washed with distilled water, eluted with 0.01M acetic acid. 
     
         __________________________________________________________________________                    Specific                          Purification        Lysozyme             Proteins                    Activity                          Sp.Act/Sp.ActFraction   ml.  Units             ng     Units/ng                          in homogenate__________________________________________________________________________Homogenate   200  3,000             11,840,000                    0.000253                          1Filtrate   200  0    11,760,000Wash    1,000        0    975,000Recovery in LysozymeInactivefractions   1,200        0    11,835,000 %           0    99.96Eluate No.1   10   250  210    1.190476                          4,7052       10   700  550    1.272727                          5,0313       10   900  700    1.285714                          5,0824       10   700  550    1.272727                          5,0315       10   300  240    1.250000                          4,9416       10   100  80     1.250000                          4,9417       10   40   30     1.333333                          5,270Recovery in LysozymeActivefractions   70   2,990             2,360 %           99.67             0.02AVERAGE ENRICHMENT IN LYSOZYME × 5,000__________________________________________________________________________ 
    
     EXAMPLE VI 
     HUMAN MONOCYTIC LYSOZYME 
     Isolation by affinity chromatography on deaminated chitin. 
     column: diameter 12 mm; height 425 mm; bed volume 48.0 ml; grain size: 200- 400 mesh. 
     Adsorption, washing and elution at constant flow: 16 cc/hour. 
     Washed with distilled water (pH 6.5), eluted with 0.01M acetic acid. 
     5 ml. Human Monocytes obtained by the Method of Archer and Kooptzoff (1958) were homogenized by sonication in 45 ml. Acetic acid 0.001M, then stirred at 4°C for 12 days prior to the application to the column. 
     
         __________________________________________________________________________                    Specific                          Purification        Lysozyme             Proteins                    Activity                          Sp.Act/Sp.ActFraction   ml.  Units             ng     Units/ng                          in homogenate__________________________________________________________________________Homogenate   50   600  1,196,000                    0.000501                          1Filtrate   50   0    1,192,000Wash    204  0    3,604Recovery in LysozymeInactivefractions   254  0    1,195,604 %           0    99.98Eluate No.1   4    44   32     1.375000                          2,7392       4    88   68     1.294110                          2,5783       4    128  92     1.391304                          2,7724       4    180  130    1.384615                          2,7645       4    108  76     1.421053                          2,8316       4    44   32     1.375000                          2,7397       4    8    15     1.333333                          2,656Recovery in LysozymeActivefractions   28   600  432 %           100  0.0004AVERAGE ENRICHMENT IN LYSOZYME × 2,726__________________________________________________________________________ 
    
     EXAMPLE VII 
     HUMAN MILK LYSOZYME 
     Isolation by affinity chromatography on deaminated chitin. 
     column: diameter 14 mm; height 444 mm; bed volume 68.3ml; grain 200- 400 mesh. 
     Adsorption, washings and elution at constant flow rate: 20 cc/hour. 
     Washed with distilled water (pH 6.6), elution with 0.01M acetic acid. 
     
         __________________________________________________________________________                    Specific                          Purification        Lysozyme             Proteins                    Activity                          Ap.Act/Sp.ActFraction   ml.  Units             ng.    Units/ng                          in whey__________________________________________________________________________Milk whey   100  7,600             3,320,000                    0.002289                          1Filtrate   100  0    3,300,000Wash    1,000        0    13,600Recovery in LysozymeInactivefractions   1,100        0    3,313,600 %           0    99.81Eluate No.1   10   480  400    1.200000                          5242       10   1,590             1,200  1.325000                          5793       10   2,400             1,800  1.333333                          5824       10   2,040             1,500  1.360000                          5945       10   720  520    1.384615                          6056       10   370  280    1.321429                          577Recovery in LysozymeActivefractions   60   7,600             5,700 %           100  0.002AVERAGE ENRICHMENT IN LYSOZYME × 577__________________________________________________________________________ 
    
     EXAMPLE VIII 
     HUMAN SALIVA LYSOZYME 
     Isolation by affinity chromatography on deaminated chitin. 
     column: diameter 10 mm; height 252 mm; bed volume 19.8 ml; grain 200-400 mesh. 
     Adsorption, washings and elution at constant flow rate: 16 cc/hour. 
     Washed with distilled water (pH 6.6), eluted with 0.01M acetic acid. 
     
         __________________________________________________________________________                    Specific                          Purification        Lysozyme             Proteins                    Activity                          Sp.Act/Sp.ActFraction   ml.  Units             ng     Units/ng                          in homogenate__________________________________________________________________________Salivahomogenate   50   2,600             184,000                    0.001413                          1Filtrate   50   0    180,000Wash    520  0    2,520Recovery in LysozymeInactivefractions   570  0    182,520 %           0    99.2Eluate No.1   10   700  520    1.296296                          9172       10   1,100             810    1.358024                          9613       10   510  400    1.275000                          9024       10   200  160    1.250000                          8855       10   80   60     1.333333                          944Recovery in LysozymeActivefractions   50   2,590             1,950 %           99.62             0.01AVERAGE ENRICHMENT IN LYSOZYME × 922__________________________________________________________________________ 
    
     EXAMPLE IX 
     HUMAN EOSINOPHYLIC LYSOZYME 
     Isolation by affinity chromatography on deaminated chitin. 
     column: diameter 12 mm; height 425 mm; bed volume 48.0ml; grain size: 200- 400 mesh. 
     Adsorption, washing and elution at constant flow: 16 cc/hour. 
     Washed with distilled water (pH 6.5), eluted with 0.01M acetic acid. 
     5 ml. Eosynophiles, obtained from human blood by the method of Lindgreen (1958), were homogenized by sonication in 25 ml. Acetic acid 0.001M, stirred for 10 days at 4°C, centrifuged and applied to the column. 
     
         __________________________________________________________________________                    Specific                          Purification       Lysozyme             Proteins                    Activity                          Sp.Act/Sp.ActFraction   ml. Units ng     Units/ng                          in homogenate__________________________________________________________________________Homogenate   30  180   1,050,000                    0.000171                          1Filtrate   30  0     1,047,000Wash    100 0     2,700LysozymeInactivefractions   130 0     1,049,700                    (99.97%)Eluate No.1   5   45    35     1.285714                          7,5192       5   100   75     1.333333                          7,7973       5   25    20     1.250000                          7,3104       5   10    75     1.333333                          7,797In LysozymeActivefractions   20  180(100%)             1,375  (0.008%)AVERAGE ENRICHMENT IN LYSOZYME × 7,606__________________________________________________________________________ 
    
     EXAMPLE X 
     HUMAN KIDNEY LYSOZYME 
     Isolation by affinity chromatography on deaminated chitin. 
     column: diameter 12 mm; height 295 mm; bed volume 33.3 ml; grain: 200-400 mesh. 
     Adsorption, washings and elution at constant flow rate: 18 cc/hour. 
     Washed with distilled water (pH 6.6), eluted with 0.01M acetic acid. 
     
         __________________________________________________________________________                    Specific                          Purification        Lysozyme             Proteins                    Activity                          Sp.Act/Sp.ActFraction   ml.  Units             ng     Units/ng                          in homogenate__________________________________________________________________________KidneyHomogenate   100  4,200             4,355,000                    0.000964                          1Filtrate   100  0    4,310,000Wash    1,020        0    40,020Recovery In LysozymeInactivefractions   1,120        0    4,350,020 %      100  0    99.89Eluate No.1   10   450  320    1.437500                          1,4912       10   810  570    1.421053                          1,4743       10   900  640    1.406250                          1,4594       10   830  590    1.406780                          1,4595       10   670  460    1.456622                          1,5116       10   360  250    1.440000                          1,4947       10   160  120    1.333333                          1,383Recovery In LysozymeActivefractions   70   4,190             2,950 %      100  99.76             0.068AVERAGE ENRICHMENT IN LYSOZYME × 1467__________________________________________________________________________ 
    
     EXAMPLE XI 
     Isolation of rabbit lung lysozyme by affinity chromatography on deaminated chitin. 
     column: diameter 12 mm; bed height 160/180 mm; bed volume 22 ml; grain: 100 mesh 
     Adsorption, washings and elution at constant flow rate: 16 cc/hour. 
     Washed with distilled water (pH 6.5), eluted with 0.1M acetic acid. 
     
         __________________________________________________________________________        Lysozyme             Protein                    SpecificFraction   ml.  Units             ng     Activity                           Purification__________________________________________________________________________Rabbit Lunghomogenate   298  6,450             5,849,740                    0.000110                           1Filtrate   298  0    5,807,420                    0Wash    3,400        0    41,600 0Eluted with0.1 Aceticacid    450  6,430             580    11,086207                           10,078 timesRecovery %   99.7__________________________________________________________________________ 
    
     EXAMPLE XII 
     Isolation of cow lung lysozyme by affinity chromatography on deaminated chitin. 
     column: diameter 12 mm; bed height 160/180 mm; bed volume 22 ml; grain: 100 mesh. 
     Adsorption, washing and elution at constant flow rate: 16 cc/hour. 
     Washed with distilled water (pH 6.5), eluted with 0.1M acetic acid 
     
         __________________________________________________________________________        Lysozyme             Proteins                    SpecificFraction   ml.  Units             ng     Activity                           Purification__________________________________________________________________________Cow Lunghomogenate   195  4,350             8,405,720                    0.000518                           1Filtrate   195  0    8,225,000                    0Wash    2,250        0    180,500                    0Elution 350  4,340             220    19,72773                           3,808Recovery %   99.77__________________________________________________________________________ 
    
     EXAMPLE XIII 
     Isolation of lettuce lysozyme by affinity chromatography on deaminated chitin. 
     column: diameter 12 mm; bed height 160/180 mm; bed volume 22 ml; grain: 100 mesh. 
     Adsorption, washings and elution at constant flow rate: 16 cc/hour. 
     Washed with distilled water (pH 6.5), eluted with 0.1M acetic acid. 
     
         __________________________________________________________________________      Lysozyme           Proteins                 SpecificFraction ml.  Units           ng    Activity                        Purification__________________________________________________________________________Homogenate 250  750  352,000                 0,002131                        1Filtrate 250  0    341,000                 0Wash  1,500      0    10,750                 0Eluate 250  745  250   1,000,000                        470Recovery % 99.33%