Ex Parte Dave et alDownload PDFPatent Trial and Appeal BoardAug 28, 201813390094 (P.T.A.B. Aug. 28, 2018) Copy Citation UNITED STA TES p A TENT AND TRADEMARK OFFICE APPLICATION NO. FILING DATE FIRST NAMED INVENTOR 13/390,094 02/10/2012 21186 7590 08/30/2018 SCHWEGMAN LUNDBERG & WOESSNER, P.A. P.O. BOX 2938 MINNEAPOLIS, MN 55402 UNITED ST A TES OF AMERICA Nitesh Dave UNITED STATES DEPARTMENT OF COMMERCE United States Patent and Trademark Office Address: COMMISSIONER FOR PATENTS P.O. Box 1450 Alexandria, Virginia 22313-1450 www .uspto.gov ATTORNEY DOCKET NO. CONFIRMATION NO. 4129.019US1 1195 EXAMINER BRADLEY, CHRISTINA ART UNIT PAPER NUMBER 1675 NOTIFICATION DATE DELIVERY MODE 08/30/2018 ELECTRONIC Please find below and/or attached an Office communication concerning this application or proceeding. The time period for reply, if any, is set in the attached communication. Notice of the Office communication was sent electronically on above-indicated "Notification Date" to the following e-mail address(es): uspto@slwip.com SLW@blackhillsip.com PTOL-90A (Rev. 04/07) UNITED STATES PATENT AND TRADEMARK OFFICE BEFORE THE PATENT TRIAL AND APPEAL BOARD Ex parte NITESH DA VE, KRISHANA CHAIT ANY A GULLA, SUND ARE SH SHANKAR, and HARISH IYER 1 Appeal2016-007333 Application 13/390,094 Technology Center 1600 Before JOHN G. NEW, TA WEN CHANG, and DAVID COTTA, Administrative Patent Judges. CHANG, Administrative Patent Judge. DECISION ON APPEAL This is an appeal under 35 U.S.C. § 134(a) involving claims to a chromatographic process for purification of a polypeptide, which have been rejected as obvious. We have jurisdiction under 35 U.S.C. § 6(b ). We AFFIRM. STATEMENT OF THE CASE Reversed-phase high-performance liquid chromatography (RP-HPLC) involves the separation of molecules on the basis of hydrophobicity. The separation depends on the 1 Appellants identify Biocon Limited as the real party in interest. (Appeal Br. 2.) 1 Appeal2016-007333 Application 13/390,094 hydrophobic binding of the solute molecule from the mobile phase to the immobilized hydrophobic ligands attached to the stationary phase, i.e., the sorbent. ... The solute mixture is initially applied to the sorbent in the presence of aqueous buffers, and the solutes are eluted by the addition of organic solvent to the mobile phase. Elution can proceed ... by gradient elution whereby the amount of organic solvent is increased over a period of time. The solutes are, therefore, eluted in order of increasing molecular hydrophobicity. ( Aguilar 9. 2) The Specification states that "usage of ion pairing agents ... in ... analytical method development and its effect on protein peak resolution is well known." (Spec. 1.) In particular, the Specification explains that, when used in RP-HPLC ion pairing agents such as trifluoroacetic acid (TFA) adsorb to the stationary phase via a hydrocarbon chain and also paired with the surface charges of a protein solute to increase the hydrophobicity of the protein. (Id. at 1-2.) The Specification further explains that, because the interaction of the ion pairing agent and protein depends on the surface charges of the protein, which differ among different proteins in a mixture, usage of the ion pairing agents results in differential binding of proteins in a mixture to the stationary phase, which in tum improves the resolution between the protein peaks as the proteins are eluted. (Id. at 2.) According to the Specification, "[h ]igher loading on the column beyond the protein injected on the column for analytical detection[] is crucial for process development and dictates the cost and yield of a given 2 Marie-Isabel Aguilar, Reversed-Phase High-Performance Liquid Chromatography, 251 METHODS IN MOLECULAR BIOLOGY, HPLC OF PEPTIDES AND PROTEINS: METHODS AND PROTOCOLS 9 (M.-I. Aguilar ed. 2004). 2 Appeal2016-007333 Application 13/390,094 process." (Id. at 2.) Further according to the Specification, the disclosures in the Specification show that "ion pairing agents have dramatic effect in the purity of proteins even after the protein loading was increased" and "demonstrates the use of ion pairing in improving yield of the chromatographic step." (Id.) Claims 1-7 and 15-19 are on Appeal. 3 Claim 1 is illustrative and reproduced below: 1. A chromatographic process for purification of a polypeptide from a mixture having at least one related impurity, at a pH ranging from about 2.5 to about 8.5, said process comprising steps of: packing RP-HPLC column with silica (C4-C18) based resin, equilibrated with about 5% to about 85 % organic modifier; loading the polypeptide mixture on the column at a flow rate of about 180 cm/hr to about 360 cm/hr; washing the column with an ion pairing agent having a concentration ranging from about 0.05% to about 1 % in combination with the organic modifier having a concentration ranging from about 5% to about 85%, at pH ranging from about 2.5 to about 8.5 and; performing a linear gradient of about 10% to about 70% of the organic modifier for eluting a purified polypeptide from the column, wherein the polypeptide is an insulin analogue of a purity ranging from about 90% to about 100% after a single chromatographic process. (Appeal Br. 15 (Claims App.).) 3 Claims 13 and 14 have been withdrawn. (Appeal Br. 4.) 3 Appeal2016-007333 Application 13/390,094 The Examiner rejects claims 1-7 and 15-19 under pre-AIA 35 U.S.C. § 103 (a) as being unpatentable over Bhopale, 4 Mills, 5 Chen, 6 Chance,7 Klyushnichenko, 8 Romanchikov, 9 Aguilar, and Grace Vydac. 10 (Ans. 2.) DISCUSSION Issue The Examiner finds that Bhopale teaches purification of recombinant insulin analogues "involv[ing] 2--4 chromatographic steps selected from reverse phase, size exclusion chromatography, hydrophobic interaction, 4 G. M. Bhopale et al., Recombinant DNA expression products for human therapeutic use, 89 CURRENT SCIENCE 614 (2005) (hereinafter "Bhopale"). 5 Janine B. Mills et al., One-step purification of a recombinant protein from a whole cell extracy by reversed-phase high-peiformance liquid chromatography, 1133 J. CHROMATOGRAPHY A 248 (2006). Page citations herein are to author manuscript version available in PMC 2009 August 6 (hereinafter "Mills"). 6 Yuxin Chen et al., Preparative reversed-phase high-peiformance liquid chromatography collection efficiency for an antimicrobial peptide on columns of varying diameters (1mm to 9.4 mm I.D.), 1140 J. CHROMATOGRAPHY A 112 (2007). Page citations herein are to author manuscript version available in PMC 2009 October 8 (hereinafter "Yuxin"). 7 Chance et al., US 5,700,662, issued Dec. 23, 1997 (hereinafter "Chance"). 8 V.E. Klyushnichenko et al., Recombinant human insulin V optimization of the reversed-phase high-performance liquid chromatographic separation, 662 J. CHROMATOGRAPHY B. 363 (1994) (hereinafter "Klyushnichenko"). 9 A.B. Romanchikov et al., Human recombinant insulin. VII. Improvement of chromatographic separation efficiency using the principle of bifunctionality, 23 BIO-ORGANIC CHEMISTRY 98 (1997) (hereinafter "Romachikov"). Page citations herein are to version in the record, apparently obtained via Infotrieve. lO Grace Vydac, THE HANDBOOK OF ANALYSIS AND PURIFICATION OF PEPTIDES AND PROTEINS BY REVERSED-PHASE HPLC (3d ed. 2002) (hereinafter "Grace Vydac"). 4 Appeal2016-007333 Application 13/390,094 charge transfer, ion exchange and affinity chromatography." (Ans. 2.) The Examiner finds that Chance, Klyushnichenko, and Romanchikov teach "the use ofRP-HPLC [reverse phase high-performance liquid chromatography] to purify insulin and its analogues, albeit in multi-step procedures." (Id. at 6.) The Examiner finds that Bhopale, Chance, Klyushnichenko, and Romanchikov do not teach a purification protocol for insulin analogues comprising RP-HPLC as the single chromatographic process. (Id. at 3, 6.) However, the Examiner finds that "Mills teaches 'a general one-step facile, flexible and readily scalable purification method for ... recombinant proteins[] based on RP-HPLC."' (Id. at 3.) The Examiner also finds that Chen teaches that "the slow acetonitrile gradients (0.1---0.2% CH3CN/min) developed by Mills for single step purification of recombinant proteins can also be used for single step purification of peptides from mixtures of close- related impurities." (Id. at 4.) The Examiner further cites Aguilar and Grace Vydac as evidence of the "high level of knowledge regarding the use of RP-HPLC for protein purification." (Id. at 7.) The Examiner concludes that a skilled artisan would have found it obvious to combine the cited prior art to arrive at the claimed invention. (Id. at 8.) In particular, the Examiner finds that a skilled artisan would have been motivated to modify Bhopale's method with the single-step RP-HPLC purification protocol taught by Mills and Chen, with a reasonable expectation of success, because Mills teaches that such single-step protocols are superior to the multi-step protocols taught by Bhopale in, e.g., purification time and yield, because Mills teaches that the one-step RP- 5 Appeal2016-007333 Application 13/390,094 HPLC protocol is a "facile, flexible and readily scalable purification method for proteins, specifically recombinant proteins," and because Mills teaches purifying a recombinant protein to 94% purity in a single step from a crude cell lysate. (Id. at 8.) As to the specific RP-HPLC conditions recited in the claims, the Examiner finds that such conditions are either disclosed by the prior art and/or are obvious to optimize through routine experimentation. (Id. at 9-- 10.) For instance, the Examiner finds that Mills, Chen, Chance, Klyushnichenko, Aguilar, Grace Vydac, and Romanchikov all teach silica based C8 resin; that Chance, Klyushnichenko, and Romanchikov all disclose purifying insulin analogues by RP-HPLC using an organic modifier (acetonitrile) in 0.1-2% ion pairing agent (trifluoroacetic acid (TFA)) at a pH within the claimed range of about 2.5 to about 8.5; that Mills and Chen teach a method of determining concentrations of acetonitrile required to elute a protein of interest, which may then be used to determine the concentration of acetonitrile in "the column equilibration mobile phase, ... the wash step, and ... the elution gradient;" and that Aguilar and Grace Vydac show a skilled artisan would have been able to "optimize both the concentration of organic modifier and ion pairing agent to achieve optimal purification" as well as the sample flow rate. (Id. at 9--10.) Appellants contend that a skilled artisan at the time of the invention "would not have expected to succeed in purifying insulin or its analogs in one step, to achieve the claimed level of purity." (Appeal Br. 8, 10-11.) 6 Appeal2016-007333 Application 13/390,094 Appellants do not separately argue the claims. 11 Accordingly, we limit our analysis to claim 1 as representative. 3 7 C.F .R. § 41.3 7 ( c )( 1 )(iv). The issue with respect to this rejection is whether a skilled artisan would have had a reasonable expectation of successfully combining the cited prior art to arrive at the invention of claim 1. Findings of Fact 1. Aguilar teaches that RP-HPLC allows for "excellent resolution ... under a wide range of chromatographic conditions for very closely related molecules." (Aguilar 9.) 2. Aguilar teaches that [ t ]he RP-HPLC experimental system for the analysis of peptides and proteins usually consists of an n-alkylsilica- based sorbent from which the solutes are eluted with gradients of increasing concentrations of organic solvent such as acetonitrile containing an ionic modifier such as trifluoroacetic acid (TF A) (1,2). Complex mixtures of peptides and proteins can be routinely separated and low picomolar-femtomolar amounts of material can be collected for further characterization. Separations can be easily manipulated by changing the gradient slope, the 11 Appellants purport to separately argue Claim 2, which depends from claim 1 and further requires that the insulin analogue be "selected from the group consisting of Aspart, Lispro, Glargine and any combination thereof." (Appeal Br. 4, 13, and 15 (Claims App.).) However, Appellants' argument with respect to claim 2 in the Appeal Brief consists solely of a statement that "the references do not render [obvious] a process geared to purify the specific insulin analogs Aspart, Lispro, Glargine, and combinations thereof, in a single chromatographic process." (Id. at 13.) Proper separate argument of a claim requires "more ... than a mere recitation of the claim elements and a naked assertion that the corresponding elements were not found in the prior art." In re Lovin, 652 F.3d 1349, 1357 (Fed. Cir. 2011). Furthermore, as the Examiner points out, Chance discloses purifying Lispro using a chromatographic process. (Ans. 6.) 7 Appeal2016-007333 Application 13/390,094 operating temperature, the ionic modifier, or the organic solvent composition. (Id. at 10; see also id. at 13 (describing the "wide range of operating parameters" that may be changed to manipulate the resolution of protein mixtures in RP-HPLC), 17 (teaching that solute retention and resolution may be manipulated through changes in the composition of the mobile phase and that proteins are routinely eluted by a gradient of increasing organic solvent concentration in RP-HPLC), 20 (choice of gradient conditions depend on nature of molecule of interest).) 3. Aguilar teaches that RP-HPLC is extremely versatile for the isolation of peptides and proteins from a wide variety of synthetic or biological sources and is used for both analytical and preparative applications .... Preparative RP-HPLC is ... used for . . . large-scale purification of synthetic peptides and recombinant proteins .... The isolation of proteins from a biological cocktail derived from a tissue extract or biological fluid for example, often requires a combination of techniques to produce a homogenous sample. HPLC techniques are then introduced at the later stages following initial precipitation, clarification, and preliminary separations using soft gels. (Id. at 11 ( citations omitted).) 4. Aguilar teaches C 18-, C4-, and CS-based sorbents are commonly employed in RP-HPLC analysis of peptides and proteins. (Id. at 13-14.) 5. Aguilar teaches that RP-HPLC is "generally carried out with an acidic mobile phase." (Id. at 17 .) 6. Agular teaches that different flow rates may be used for columns of different sizes in RP-HPLC. (Id.) 8 Appeal2016-007333 Application 13/390,094 7. Grace Vydac teaches that RP-HPLC "has become a widely used, well-established tool for the analysis and purification of biomolecules" because it is able to "separate polypeptides of nearly identical sequences, not only for small peptides ... but even for much larger proteins." (Grace Vydac 2.) 8. Grace Vydac teaches that "[p ]olypeptides which differ by a single amino acid residue can often be separated by RP-HPLC" and that "most variants [ of insulin] can be separated by RP-HPLC" even though "[i]nsulin variants have molecular weights of around 5,300 with only slightly different amino acid sequences." (Id.) 9. Grace Vydac teaches using RP-HPLC to separate rabbit and human insulin, which differs only by a single amino acid, using a silica C4 column and an eluent of 27-30% acetonitrile in 0.1 % TF A over 25 minutes at 1.5 mL/minute. (Id.) 10. Grace Vydac teaches that, in RP-HPLC, polypeptides adsorb to the surface of the hydrophobic stationary phase after entering the HPLC column and remain adsorbed until the concentration of organic modifier reaches the critical concentration necessary to cause desorption. (Id. at 4.) More particularly, Grace Vydac teaches that [ t ]he desorption and elution of polypeptides from RP HPLC columns is accomplished with aqueous solvents containing an organic modifier and an ion-pair reagent or buffer. The organic modifier solubilizes and desorbs the polypeptide from the hydrophobic surface while the ion- pair agent or buffer sets the eluent pH and interacts with the polypeptide to enhance the separation. Elution is accomplished by gradually raising the concentration of organic solvent during the chromatographic nm (solvent gradient). When the solvent reaches the precise 9 Appeal2016-007333 Application 13/390,094 concentration necessary to cause desorption, the polypeptide is desorbed and elutes from the column. (Id. at 17.) 11. Grace Vydac teaches that "[ t ]he sensitivity of polypeptide desorption to precise concentrations of organic modifier accounts for the selectivity of RP-HPLC in the separation of polypeptides." (Id. at 5; see also id. at 6 (teaching that "polypeptides are very sensitive to organic modifier concentration).) 12. Grace Vydac teaches that gradient elution is usually preferred over isocratic elution in RP-HPLC and that "[s]lowly raising the concentration of organic solvent results in the sharpest peaks and best resolution." (Id. at 6, 18 ( emphasis omitted).) Grace Vydac recommends "beginning gradients at no less than 3 to 5% organic modifier concentration" and "ending gradients at no more than 95% organic modifier." (Id. at 18.) 13. Grace Vydac teaches that TFA is widely used as an ion-pairing agent and that it is normally used at concentrations of about 0.1 % (w/v). (Id. at 19. Grace Vydac further teaches that, [ a ]lthough TF A is typically present in the mobile phase at concentrations of 0.05% to 0.1 %, varying the concentration of TF A has a subtle [ e ]ffect on peptide selectivity .... This means that, for good reproducibility, it is important to control the TF A concentration very carefully in peptide separation methods. This provides another tool for optimizing peptide resolution. After the column and gradient conditions have been selected, it is possible to vary the TF A concentration slightly to further optimize resolution between peptide pairs. (Id. at 20.) 10 Appeal2016-007333 Application 13/390,094 14. Grace Vydac teaches that "[p ]eptide separations are often sensitive to the eluent pH" and that pH "can be a useful tool in optimizing peptide separations." (Id. at 22.) 15. Grace Vydac teaches that, while protein resolution is relatively independent of mobile phase flow rate, flow rate may influence aspects of a separation such as detection sensitivity, sample solubility, column back- pressure, and gradient slope and shape. (Id. at 24--25.) 16. Grace Vydac teaches that "[p]reparative RP-HPLC is frequently used to purify synthetic peptides in milligram and gram quantities." (Id. at 3; see also id. at 40 (explaining that RP-HPLC is used to purify microgram to milligram quantities of polypeptides for research purposes as well as to purify up to gram quantities of recombinant proteins for use in clinical trials or for marketed products).) 1 7. Grace Vydac teaches that scaling up laboratory separations to process scale may involve increasing the size of the column and elution flow rate, a change in elution solvents, use of different ion-pairing agents or buffers, and/or a change in gradient conditions. (Id. at 40; see also id. at 42.) 18. Bhopale teaches that "[ r ]ecombinant DNA (rDNA) technology has made a revolutionary impact in the area of human healthcare by enabling mass production of safe, pure and effective rDNA expression products" and that, "[ c ]urrently, several categories of rDNA products, viz. hormones of therapeutic interest ... are being produced using rDNA technology for human use." (Bhopale Abstract (emphasis omitted).) 19. Bhopale teaches a general process for purification ofrDNA products. (See, e.g., id. at Fig. 2.) Bhopale teaches that, while "[t]here are several different methods that can be used for purification of rDNA 11 Appeal2016-007333 Application 13/390,094 products,[] only chromatographic purification methods are generally used." (Id. at 616.) Bhopale teaches that "[a] combination of two to four different chromatographic techniques is generally employed in a typical downstream processing procedure." (Id.) Bhopale teaches reversed phase (RP) chromatography as one of the chromatographic purification methods used for rDNA products. (Id. at 616 (Table 1).) 20. Bhopale teaches human insulin, insulin aspart, insulin glargine, insulin lispro, and insulin glulisine as some of the "important rDNA products ... approved by FDA for human therapeutic use." (Id. at 617 (Table 2); see also id. at 618---619 ( describing use of human insulin produced using S. cerevisae or E. coli to treat diabetes mellitus).) 21. Romanchikov studies the retention mechanisms of insulin and an analog in RP-HPLC. (Romanchikov Abstract.) 22. Romanchikov teaches that separation selectivity and resolution of these proteins were dependent on the composition and properties (e.g., salt buffer type, pH, ionic strength) of the mobile phase and also teaches that separation selectivity may be "regulated by altering the contribution of each of the two separation mechanisms," (i.e., interaction with the hydrophobic and the ion-exchange groups on the silica gel). (Id.; see also id. at 3, 7, 9-- 10, and Fig. 3.) 23. Romanchikov teaches that the concentration and size of hydrophobic section of the ion pairing agent also influence insulin retention. (Id. at 7.) 24. Romanchikov illustrates the dependence of insulin retention coefficient on salt concentration using a column with silica (C8) based resin (Armsfer-Si-100 Cs (PR)) and mobile phases comprising an organic 12 Appeal2016-007333 Application 13/390,094 modifier and ion pairing agent (20% acetonitrile (CH3CN) and 0.3% TFA, or 16.2% acetonitrile and 0.1 % TFA). (Id. at Fig. 4.) 25. Romanchikov illustrates the dependence of the insulin retention coefficient on ion pairing agent concentration in mobile phase using a column with silica (C8) based resin (Armsfer-Si-100 Cs (PR)) and mobile phases comprising an organic modifier (16.6% or 22.4% acetonitrile) and an ion pairing agent (0.1 o/o--0.5% TFA or heptafluorobutyric acid (HFBA)). (Id. at Fig. 5.) 26. Romanchikov illustrates the dependence of the insulin retention coefficient on organic modifier concentration using a column with silica (C8) based resin (Armsfer-Si-100 Cs (PR)) and mobile phases comprising acetonitrile as the organic modifier and 0.1, 0.3, or 0.5% TFA or HFBA as ion pairing agent. (Id. at Fig. 6.) 27. Romanchikov teaches separation of insulin and its analog (deamido insulin) using a column with silica (C8) based resin (Armsfer- Si - 100 Cs (PR)) in gradient mode. (Id. at Fig. 7.) 28. Romanchikov teaches that"[ o Jptimal parameters of reverse- phase system were found for effective separation of insulin and deamido insulin on bifunctional sorbent both for analysis as well as for preparative obtaining of highly purified insulin" and further teaches that "[k ]nowing the interaction mechanisms of proteins with mobile and stationary phases has given new possibilities to control the main characteristics of chromatographic process - separation selectivity coefficient and resolution capability of system[-] by changing the parameters of mobile and stationary phases." (Id. at 10.) 13 Appeal2016-007333 Application 13/390,094 29. Klyushnichenko relates to the applicability of RP-HPLC to analysis of the products of recombinant insulin and investigates the "influence of several mobile phases in reversed-phase ... HPLC on selectivity, resolution and sensitivity." (Klyushnichenko Abstract; see also id. at 364, left column.) 30. Klyushnichenko teaches establishing optimum conditions for separation of insulin-related proteins on commercial and laboratory-made supports via optimization of selectivity and resolution as a function of pH and ionic strength. (Id.; see also id. at 366-367, and 368-369 (optimization for scaling up).) 31. Klyushnichenko teaches that, "[i]n spite of small differences in the structure and sequence of animal and human insulin, RP-HPLC ensures the separation of these proteins and their derivatives and precursors. The flexibility of this method is demonstrated by the quality of the separation of insulin, proinsulin and desamidinsulin peaks." (Id. at 363, right column ( citations omitted).) 32. Klyushnichenko teaches that "HPLC is an effective method not only for analytical separations, but also for the preparative isolation of insulin with high purity." (Id. at 364, left column.) 33. Klyushnichenko illustrates separation of recombinant insulin by HPLC using various columns with silica based resin (C4-C18). (Id. at 364, left column.) 34. Klyushnichenko illustrates separating insulin and its analog using mobile phases comprising 10% acetonitrile-0.1 % TF A and 100% acetonitrile-0.1 % TFA. (Id. at Fig. 2, Fig. 5.) 14 Appeal2016-007333 Application 13/390,094 35. Klyushnichenko concludes that its proposed techniques "ensures a high quality of active insulin production." (Id. at Abstract.) 3 6. Chance teaches "[ r ]ecombinant processes for preparing insulin analogs modified at position 29 of the B-chain and, optionally, at other positions." (Chance Abstract.) 3 7. Chance teaches that a particularly preferred insulin analog of its invention is "one wherein B28 is lysine and B29 is proline, i.e., an inversion of the native human insulin amino acid sequence at positions 28 and 29 of the B-chain." (Id. at 3:49-52; see also id. at Example 1 (Lys(B28), Pro(B29) Human Insulin).) 38. Chance teaches purifying a sample of an insulin analog (Lys(B28), Pro(B29) human insulin) as follows: Th[ e] sample was further purified by reverse-phase HPLC (using a 2.12x25 cm DuPont C8 column eluted at room temperature, at 2.6 ml/min, using a linear gradient of increasing acetonitrile in O. IM NaH2P04, pH 2.2). The effluent was monitored at 2 7 6 nm. Selected fractions were assayed by analytical HPLC. The desired fractions were pooled and further purified using pH 7 HPLC as follows. The pool from the low pH HPLC preparation run was diluted approximately 2 times in an ice bath with O. IM (NH4)2HP04. The pH was adjusted to 7 with cold 2NNaOH in an ice bath. The sample was loaded onto and eluted from the same HPLC column using the same conditions as the low pH preparation run except the eluting buffer was O. IM, pH 7 (NH4)2HP04/acetonitrile. The pool from the pH 7 HPLC preparative run was chilled in an ice bath and diluted two times with 0.1 % aqueous trifiuoroacetic acid (T'FA). IN HCl was added (cold, sample in ice bath) to lower the pH to 3. The sample was loaded onto a Vydac C4 or, alternatively a DuPont C8 HPLC column (2.12x25 cm) and eluted with a linear gradient of increasing acetonitrile in 0.1 % aqueous TFA. 15 Appeal2016-007333 Application 13/390,094 The effluent was monitored at 214 nm or 276 nm. The desired fractions were pooled and lyophilized giving a sample yield of 41 mg of the desired analog of greater than 97 percent purity by reverse-phase HPLC. (Id. at 9: 1-25.) 39. Chance also teaches eluting an insulin analog using linear gradient of increasing acetonitrile in 0.1 % or 0.5% TF A using a C-8 Ultrasphere HPLC column or a C-18 Vydac column. (See e.g., id. at 9:55- 59, 10:24--28, 10:50-54, 11:8-14, 11:34--38, 11:61---63, 13:12-21, 13:51-55, 14:10-14, 14:36-40, 14:62---66, 15:20-24, 15:46-50, 16:4--8, 16:29-33, 16:54--58, 17: 11-15, 17:37--41, 17:63---67, 18:22-26, 18:48-52, 19:6-10, 19:29-33, 19:54--58, 20: 11-15, 42:51-56, 43:61---65, 44:40--45, 46: 1---6; see also id. at 43:29--41 (purifying insulin analog using C-18 Vydac HPLC column, washing with a buffer consisting of 10 parts acetonitrile and 90 parts 0.5% TFA solution (buffer A), applying a linear gradient from 0-20% of a buffer consisting of 50 parts acetonitrile and 50 parts 0.5% TFA (buffer B) at 2.4 ml/min, and applying a linear gradient of 20-70% of buffer Bat 8 ml/ min).) 40. Mills teaches that both affinity and immunoaffinity chromatography techniques are often critical in developing purification procedures for recombinant proteins, often as the first step in a multicolumn purification approach. . . . Although multicolumn protocols (generally employing combinations of affinity, ion-exchange and size-exclusion chromatography) are effective[], complications remain ... leading to an increase in purification time as well as a concomitant loss of purified sample yield. Further, even if a one-step affinity approach to purification of a protein on a small scale was favoured, scale-up to larger sample amounts may become prohibitively expensive. 16 Appeal2016-007333 Application 13/390,094 (Mills 1 ( citations omitted).) 41. Mills teaches "a one-step facile, flexible and readily scalable purification method for a recombinant protein, TM 1-99 ( 113 amino acid residues; 12,837 Da) based on reversed-phase high-performance liquid chromatography (RP-HPLC) from an E. coli cell lysate." (Mills Abstract.) 42. Mills describes carrying out its method on a Zorbaz 300SB-C8 column. (Id. at 2.) 43. Mills teaches performing analytical and preparative RP-HPLC under the following conditions: 2.4.1. Analytical RP-HPLC-Analytical runs and fraction analyses were carried out by a linear AB gradient (1 % B/min for analytical profiles and 2% B/min for fraction analysis) at a flow-rate of 0.3 ml/min where Eluent A is 0.05% aq. TFA and Eluent B is 0.05% TFA in acetonitrile; temperature, 25 °C. TF A concentrations of 0.05---0.1 % are characteristic of most separations of peptides and proteins by RP- HPLC (for both analytical and scale-up purposes[)]. .... 2.4.2. Preparative RP-HPLC-Preparative purification was carried out by a linear AB gradient (Eluent A is 0.05% aq. TFA, pH 2.0, and Eluent Bis 0.05% TFA in acetonitrile) of 2% B/min up to 24% B, followed by a slow (0.1 % B/min) gradient up to 40% B. A rapid rise (4% B/min) up to 60% B was then followed by an isocratic wash with 60% B .... Flow-rate, 0.3 ml/min; temperature, 25 °C (Id. at 3.) 44. Mills teaches that "[a] key advantage of [its] slow gradient approach is the high sample loading concentrating the desired material on the column, thus aiding its separation from closely adjacent impurities." (Id. at 4.) Mills further teaches that another advantage of its method is that "the slow gradient spreads the desired product over a large number of fractions, the bulk of which would contain purified product only, with just the first and 17 Appeal2016-007333 Application 13/390,094 last product fractions containing hydrophilic and hydrophobic impurities, respectively." (Id.) 45. Mills teaches a "'rule of thumb' approach whereby the shallow gradient is started 15% below the acetonitrile concentration required to elute the protein of interest in an analytical run can be applied as a general rule of thumb for polypeptides of IO-residue length and longer." (Id.) Mills teaches that this rule is based on the fact that "peptides and proteins exhibit only narrow partitioning windows," has the advantage of being able to separate a large range of sample loads, and "is a good compromise between the time taken for efficient product purification and obtaining maximum sample load, i.e., a lower or greater starting acetonitrile concentration would extend the run time or decrease maximum sample load, respectively." (Id. at 4--5.) 46. Mills teaches that, using its method, "[l]oads of 23 and 48 mg of lyophilized crude cell extract produced 2.4 and 4.2 mg of purified product (>94% pure), respectively." (Id. at Abstract.) Mills states that its results "show the excellent potential of one-step RP-HPLC for purification of recombinant proteins from cell lysates, where high yields of purified product and greater purity are achieved compared to affinity chromatography." (Id.) 47. Mills concludes that "a one-step RP-HPLC slow gradient approach shows excellent potential for purification of recombinant proteins from cell lysates, where high yields of purified product are achieved compared to affinity chromatography." (Id. at 6.) 48. Chen teaches that "[t]o obtain antimicrobial peptides, peptide synthesis is the favored method especially for de nova antimicrobial peptide design," but "[t]he impurities created during peptide synthesis are usually 18 Appeal2016-007333 Application 13/390,094 closely related structurally to the peptide of interest and hence often pose difficult purification problems." ( Chen 1; see also id. at 4 ( describing antimicrobial peptide used in the study and stating that "both hydrophilic and hydrophobic impurities are present in the crude peptide mixture, a number of which are eluted close to the peptide of interest").) 49. Chen teaches that [t]he excellent resolving power of reversed-phase high- performance liquid chromatography (RP-HPLC) has made it the predominant high-performance liquid chromatography (HPLC) technique for preparative peptide separations. Indeed, not only is RP-HPLC usually superior to other modes of HPLC with respect to both speed and efficiency, but it also offers the widest scope for manipulation of mobile phase conditions and choices of different columns to optimize separations. (Id. at 1 ( citations omitted).) 50. Chen describes "the application of a one-step preparative RP- HPLC protocol employing slow acetonitrile gradients to the purification of an amphipathic, a-helical antimicrobial peptide on reversed-phase columns of varying column diameters (1 mm to 9.4 mm I.D.)." (Id. at 2.) Chen teaches that one-step RP-HPLC purification procedures may avoid loss of product yield, "which is frequently a feature of multi-step protocols." (Id.) 51. Chen's study was conducted using columns with silica (C8) based resin. (Id. at 3, 5.) 52. Chen teaches the following HPLC conditions for its study: All preparative runs were carried out with a linear AB gradient (1 % acetonitrile/min for 30 min up to 30% acetonitrile, followed by 0.1 % acetonitrile/min for 250 min up to 55% acetonitrile) at room temperature and a flow-rate of 2 ml/min, 1 ml/min, 0.25 ml/min or 0.08 ml/min for the semi-preparative column, analytical 19 Appeal2016-007333 Application 13/390,094 column, narrowbore column and micro bore column, respectively, where eluent A was 0.2% aq. trifluoroacetic acid (TFA) pH 2 and B was 0.2% TFA in acetonitrile. Chen et al. had previously demonstrated that 0.2---0.25% TF A in the mobile phase achieved optimum resolution of peptide mixtures compared to the 0.05---0.1 % TFA concentrations traditionally employed. Following the slow gradient step, the column was washed with 70% acetonitrile for 3 0 min. All samples were loaded at the same flow-rate as the flow- rate used for column elution. Analytical RP-HPLC was carried out on the Zorbax 300 SB-Cs narrowbore column with a linear AB gradient (1 % acetonitrile/min) at a flow-rate of 0.25 ml/min, where eluent A was 0.2% aq. TFA, pH 2, and eluent B was 0.2% TF A in acetonitrile. (Id. (citation omitted).) 53. Chen teaches that, "[i]n order to design a slow gradient preparative protocol, it is first necessary to determine the concentration of acetonitrile required to elute the peptide of interest during an initial analytical run" and that, to establish the percentage acetonitrile at which the 0.1 % acetonitrile/min slow gradient should begin, the "rule of thumb" for polypeptides of 10 residues in length and longer is to "start at an acetonitrile concentration 12% below that required to elute the peptide in the 1 % acetonitrile/min analytical run." (Id. at 5.) 54. Chen teaches that [a] key advantage of such a slow gradient approach is that, at high sample loads, sample displacement can occur 20 Appeal2016-007333 Application 13/390,094 (Id.) where the hydrophobic impurities displace the product of interest and the product of interest displaces the hydrophilic impurities during partitioning of product and impurities, thus, aiding in the separation of product from closely adjacent impurities. [] In addition, the desired product may be eluted over a number of fractions, the bulk of which would contain purified product only, with just the first and last product fractions containing hydrophilic and hydrophobic impurities, respectively, leading to improved resolution and yield of the product of interest. 5 5. Chen teaches that "excellent product purity (>99%) and yield" was obtained by its slow gradient approach to purification of the 200 mg sample load using the semi-preparative column. (Id. at 6.) 56. Chen teaches that a recombinant protein (114 amino acid residues) of >94% purity was obtained using its one-step slow gradient protocol. (Id. at 8.) 57. Chen states that one of its objectives is "to examine the potential of [a] slow gradient protocol as a general method for purifying peptides with closely-related impurities from a wide range of sample loads." (Id. at 2; see also id. at 5 (stating that "it is our intent to make [a] purification protocol generally applicable to polypeptides in general") and 6 ( explaining that the slow gradient approach is effective for resolution of desired peptide product from even closely structurally related synthetic purities because "only one fraction for each sample load contained overlapping product and hydrophilic impurities of any significance").) Chen teaches that its "straightforward one-step slow gradient protocol shows excellent potential as a universal method for purification of synthetic peptides with closely structurally related impurities." (Id. at 9; see also id. at Abstract.) 21 Appeal2016-007333 Application 13/390,094 Analysis Except as otherwise noted, we adopt the Examiner's findings, analysis, and conclusions with respect to claim 1, including with regard to the scope and content of, and motivation to modify or combine, the prior art, as set forth in the Final Action and Answer. (Final Act. 2-11, 12-15; Ans. 2-10, 11-27, FF1-FF57.) We address Appellants' arguments below. Appellants concede that RP-HPLC "and other separation techniques have been used to purify proteins in general, even at [the] preparative scale," and that "insulin or its analogs could be purified to a high level of purity using RP-HPLC." (Appeal Br. 12.) However, Appellants contend that a skilled artisan at the time of the invention "would not have expected to succeed in purifying insulin or its analogs in one step, to achieve the claimed level of purity." (Id. at 8, 10-11.) More particularly, Appellants contend that: (1) "one cannot ... generalize a one-step purification of prior art proteins that are in no way related to insulin or its analogs, to the purification of the claimed proteins" (id. at 8, 11-12), and (2) the Examiner "appears to ignore the stark differences between separation methods developed for analytical scale and those developed for preparative scale." (Id. at 8, 12- 13.) We are not persuaded. With respect to Appellants' argument that the one-step RP-HPLC method references such as Mills and Chen cannot be generalized to the purification of insulin analogs, we agree with the Examiner that a skilled artisan would have a reason for, as well as a reasonable expectation of success in, adapting the one-step method taught by Mills and Chen to purify insulin, given that: (1) references such as Bhopale teach the desirability of purifying insulin analogs from related impurities; (2) 22 Appeal2016-007333 Application 13/390,094 "Mills and Chen successfully appl[ied] the single[-step] RP-HPLC method to proteins that are different from insulin but are also very different from each other, underscoring the versatility of the approach"; and (3) references such as Grace Vydac show that there is high level of skill and knowledge in the art such that HPLC conditions are routinely optimized for protein purification. (Ans. 12, 21-22.) We further note that Chen explicitly states that its one-step purification protocol "shows excellent potential as a universal method for purification of synthetic peptides with closely structurally related impurities." (FF57 ( emphasis added).) Appellants contend in the Reply Brief that "Bhopale published very close in time to Chen and Mills" and that "Bhopale strongly suggests that at about the same time that Mills and Chen [were] conducting their purification on proteins wholly unrelated to the claimed proteins, those of ordinary skill in the art would have at best expected a multi-step purification process to purify the claimed protein." (Reply Br. 2-3.) Appellants similarly cite Chance as suggesting that a skilled artisan would have expected multi-step purification process to be required for purifying insulin analogs. (Id. at 3.) We are not persuaded. Appellants base their argument on Bhopale and Chance but do not sufficiently take Chen, Mills, and other cited references into account. 12 However, "[ n ]on-obviousness cannot be 12 Appellants contend that 'just because Chen and Mills were lucky in purifying proteins wholly unrelated to the claimed proteins does not necessarily mean that those of ordinary skill in the art would have had the reasonable expectation of success in purifying the claimed proteins at the claimed level of purity." (Reply Br. 3.) We are not persuaded for the reasons already discussed above. Chen and Mills do not suggest that the results of their purification methods are a matter of luck. Likewise, we emphasize that, for purposes of an obviousness analysis, "expectation of 23 Appeal2016-007333 Application 13/390,094 established by attacking references individually where the rejection is based upon the teachings of a combination of references." In re Merck & Co., 800 F .2d 1091, 1097 (Fed. Cir. 1986). Instead, the references "must be read, not in isolation, but for what [they] fairly teach[] in combination with the prior art as a whole." Id. We agree with the Examiner that Bhopale and Chance, when read in combination with Chen and Mills, provide a skilled artisan with a reasonable expectation of success in arriving at a one-step chromatographic process for purifying insulin analogs. As to Appellants' argument that the prior art relates to purification methods on the analytical scale, we note as does the Examiner that the claim is not limited to purification on a preparative scale. (Ans. 20.) Furthermore, even assuming the claim requires purification on a preparative scale, a skilled artisan would have a reasonable expectation of success in combining the cited references to arrive at the claimed purification method on such a scale. As the Examiner points out, Mills teaches that its one-step purification process is readily scalable, Chen provides examples wherein 100 mg and 200 mg of peptides are purified and further describes its method as a "one-step slow gradient preparative protocol," and Grace Vydac suggests that a skilled artisan would be able to scale up laboratory separations to process scale separations by adjusting particular HPLC conditions. (Ans. 20, 24--25; FFl 7; FF41; Chen Fig. 4 and Abstract.) Finally, to the extent Appellants argue that the subject matter of claim 1 exhibits unexpected results, we are not persuaded. In particular, Appellants argue that the results achieved by the method of claim 1 is success need only be reasonable, not absolute." Pfizer, Inc. v. Apotex, Inc., 480 F.3d 1348, 1364 (Fed. Cir. 2007). 24 Appeal2016-007333 Application 13/390,094 "unexpected based on Bhopale' s teachings" and that "[ t ]he claimed process is ab initio 'superior to the procedures in the art' because it achieves a result that has never been described in the art." (Reply Br. 3; see also id. at Appeal Br. 8.) Once again, however, Appellants attack a reference (Bhopale) individually without taking into account the combination of cited references including Chen and Mills. Likewise, the fact that the result of a claimed method is superior or has not previously been described in the art does not automatically render the result unexpected, particularly in the context of an obviousness rejection. Pfizer, Inc. v. Apotex, Inc., 480 F.3d 1348, 1371 (Fed. Cir. 2007) (explaining that a superior property must still be unexpected to be considered evidence of non-obviousness). Appellants argue in the Reply Brief that - contrary to the Examiner's contention that Appellants have not established unexpected results because the examples in the Specification do not sufficiently describe the contents of their starting materials (Ans. 16-18)-the examples in the Specification identify at least some impurities in Appellants' starting materials. (Reply 3- 4.) While we agree with Appellants that the examples appear to identify at least some of the impurities present in their starting materials, we also agree with the Examiner's broader point that Appellants have not persuasively shown that the presence of the particular impurities in the starting samples render the result of the purification process unexpected. Moreover, the Examiner finds that the data supplied by the examples in the Specification are not commensurate with the broad scope of the claim, as required by a showing of unexpected results. (Ans. 16-18.) In the Reply Brief, Appellants contend that the Specification describes purification results for insulin analogs Aspart, Lispro, and Glargine and that they thus "have 25 Appeal2016-007333 Application 13/390,094 shown that a sufficient number of species encompassed by the claimed genus demonstrate the unexpected results." (Appeal Br. 4.) We are not persuaded by Appellants' argument. Appellants fail to provide persuasive evidence or explanation why Aspart, Lispro, and Glargine are sufficiently representative of insulin analogs to render the examples in the Specification commensurate with the scope of claim 1. "Attorneys' argument is no substitute for evidence." Johnston v. IVAC Corp., 885 F.2d 1574, 1581 (Fed. Cir. 1989). In addition, claim 1 encompasses a wide variety of types of impurities, organic modifiers, ion pairing agents, and HPLC conditions. Thus, assuming that Aspart, Lispro, and Glargine are representative of insulin analogs, Appellants still fail to explain how the examples in the Specification provides evidence of unexpected results commensurate with the scope of the claim. For this additional reason, we are not persuaded that the alleged unexpected results proffered by Appellants demonstrate the process of claim 1 to be non- obvious.13 Finally, Appellants contend that the rejection is based on impermissible hindsight. (Reply Br. 5.) We are not persuaded. "Any judgment on obviousness is in a sense necessarily a reconstruction based 13 Appellants further argue that, even if the data in the Specification is not commensurate with the scope of claim 1, the same would not be true of claim 2. (Reply Br. 4--5.) As we noted earlier, however, Appellants did not properly separately argue claim 2 in the Appeal Brief. See supra note 11. In any event, as discussed above, while claim 2 limits the insulin analog to the group consisting of Aspart, Lispro, Glargine, and combinations thereof, Appellants have neither shown that the results achieved by the claimed method is unexpected in the first place, or that the data provided in the Specification shows unexpected results commensurate with the scope of other limitations in claim 2. 26 Appeal2016-007333 Application 13/390,094 upon hindsight reasoning, but so long as it takes into account only knowledge which was within the level of ordinary skill at the time the claimed invention was made and does not include knowledge gleaned only from applicant's disclosure, such a reconstruction is proper." In re McLaughlin, 443 F.2d 1392, 1395, 170 USPQ 209,212 (CCPA 1971). For the reasons already discussed, we find that the Examiner's rejection of claim 1 is properly based on the knowledge within the level of ordinary skill at the time of the claimed invention, as evidenced by the cited prior art, rather than any knowledge gleaned only from Appellants' disclosure. Accordingly, we affirm the Examiner's rejection of claim 1. Claims 2-7 and 15-19, which are not separately argued, fall with claim 1. 37 C.F .R. § 41.3 7 ( c )(1 )(iv). SUMMARY For the reasons above, we affirm the Examiner's decision rejecting claims 1-7 and 15-19. TIME PERIOD FOR RESPONSE No time period for taking any subsequent action in connection with this appeal may be extended under 37 C.F.R. § 1.136(a). AFFIRMED 27 Copy with citationCopy as parenthetical citation
