TREA

Process for the preparation of compounds with enhanced optical purity

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Information

  • Patent Grant
  • 7129059
  • Patent Number
    7,129,059
  • Date Filed
    Wednesday, February 8, 2006
    18 years ago
  • Date Issued
    Tuesday, October 31, 2006
    17 years ago
Information
Abstract
A process for preparation of a compound with enhanced optical purity is disclosed wherein a mixture of the enantiomers of a chiral amine is brought into contact with an enzyme having peptide deformylase activity with a bivalent metal ion as a cofactor.
Description

The invention relates to a process for the preparation of a compound with enhanced optical purity wherein a mixture of the enantiomers of a chiral compound of formula 1:




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wherein:

  • R1 represents an optionally substituted alkyl or an optionally substituted aryl group
  • R2 represents H, an optionally substituted alkyl or an optionally substituted aryl group
  • Y represents an alkyl group, an aryl group, (CH2)nCOOH, (CH2)n—COOR, (CH2)n—CONRR′, CH2OH, or C≡N wherein R and R′ independently represent H, an alkyl or aryl group, and n represents 0 or 1, is brought into contact with an enzyme having peptide deformylase activity with a bivalent metal ion as a cofactor wherein the metal is chosen from the groups 5–11 of the periodic system.


Enzymes having peptide deformylase activity are known in the literature e.g. from P. T. Ravi Rajagopalan et al., Biochemistry 1997, 36, 13910–13918 wherein the use of peptide deformylase is described for the deformylation of several peptides with N-formylmethlonine at the N-terminus and of N-formylmethionine. Although the known peptide deformylases showed reasonable deformylase activity when peptides where used as a substrate, they showed no or little activity with respect to N-formylmethionine.


Applicant surprisingly found that the peptide deformylases having a bivalent metal ion as a cofactor according to the invention, did not only show a considerable activity towards the substrates according to formula 1, but also appeared to be enantioselective. U.S. Pat. No. 4,745,067 discloses L-aminoacylases which exhibit enantioselective activity towards N-acyl-L-amino acids. However, the activity of these enzymes towards N-formyl-L-methionine is low.


The alkyl groups in R1, R2, R, R1 en Y may be cyclic or linear or branched chains. The alkyl, aryl and the methylene groups may be substituted Suitable substituents are for instance, hydroxy, alkyl, alkoxy, e.g. methoxy, mercapto, alkylmercapto, amino, guanyl, carboxamide, halogen, e.g. chloro, aryl, e.g. phenyl and hydroxyphenyl, imidazolyl or indonyl.


Substrates according to formula 1 that can be used in the process of the invention are for instance amino acids, for instance α- or β-amino acids with 1–20 C-atoms, In particular α-H-α-amino acids, α-methyl-α-amino acids, β-amino acids; esters of said amino acids wherein the ester group is for instance an alkyl group having 1–10 C-atoms; amides of said amino acids, wherein optionally the amide is N-substituted with 1 or 2, preferably 1, substituent chosen from alkyl or aryl, having 1–10 C-atoms; nitriles corresponding to said α-amino acids; amino alcohols corresponding to said α-amino acids; or amines for instance (optionally substituted) aromatic or aliphatic amines. Suitable substituents are for instance (optionally substituted) alkyl groups, for instance with 1–10 C-atoms.


In another embodiment of the present invention a mixture of the enantiomers of a (non protected) amino compound is subjected to a formylation in the presence of a peptide deformylase having a bivalent metal ion as a cofactor, wherein the metal is chosen from the groups 5–11 of the periodic system and a formylating agent, whereby one of the enantiomers is selectively converted into the corresponding N-formyl amino compound.


Suitable formylating agents are for instance formic acid in case a thermodynamically controlled formulation can be performed, or formic acid esters or amides when the formulation is kinetically controlled. In a thermodynamically controlled formylation the equilibrium is shifted towards the side of formyl derivative, preferably by precipitation of the formyl derivative.


Peptide deformylases are in general enzymes having formyl methionine peptide deformylase activity. The peptide deformylases to be used according to the invention have a more than 10 times, preferably more than 100 times, in particular more than 1000 times, higher activity towards the formyl protected compounds according to formula 1 compared to the corresponding acetyl protected compounds. Activity here is defined as the catalytic efficiency (also called: specificity constant) Kcat/Km expressed in M−1 sec−1; wherein Km (expressed in mM) represents the Michaelis constant (this is the substrate concentration at which the reaction rate is 50% of the maximum reaction rate observed) and Kcat (expressed in min−1) represents the turnover number. It should be noticed that in the literature also other names are being used instead of the name Peptide deformylases; in particular the following names may be mentioned here: formylmethionine deformylase, N-formylmethionyl aminoacyl-tRNA deformylase, N-formyl-L-methionine amidohydrolase N-formylmethionyl-aminoacyl-tRNA amidohydrolase.


Suitable peptide deformylases to be used in the process according to the invention are peptide deformylases classified as EC 3.5.1.27. Preferably, the enzyme is an enzyme having the activity as described for EC 3.5.1.27 because excellent results are being achieved in the deformylation with such enzymes. It should be noticed, that until recently it was believed that the enzyme coded as EC 3.5.1.31 is catalyzing a different reaction. In the meantime however it has been shown that the enzymes known as EC 3.5.1.27 and EC 3.5.1.31 are coded for by exactly the same gene and have the same activity. Therefore, as used herein, the term EC 3.5.1.27 is encompassing not only EC 3.5.1.31, but likewise all other enzymes having the same activity as described for EC 3.5.1.27.


Although the family of PDF's is composed of proteins with a relatively low level of sequence identity, the 3D structures of the members of this family appear closely related one to each other with, in particular, the building of a common fold around the bivalent metal ion and three signature sequences. As is described (for PDF's indicated as PDF) by Wagner et al., J. Biol. Chem., 273, 11413–6 (1998), for many of these enzymes characteristically three short amino acid stretches are present as strictly conserved motifs, namely in that the enzymes contain the sequences (i) HEXXH, (ii) EGCLS and (iii) GXGXAAXQ. In these sequences X represents any natural amino acid, and standard one letter codes for amino acids are used: A=alanine, C=cysteine, E=glutamic acid, G=glycine, H=histidine, L=leucine, S=serine and Q=glutamine.


Peptide deformylases are obtainable for instance from eubacteria for example Escherichia coli, Bacillus subtilis, Clostridium acetobutylicum Clostridium beyerinckii, Haemophilus influenzae Thermotoga maritima, Thermus aquaticus, Thermus thermophilus, Calothrix PCC 7601, Bacillus stearothermophilus or Lactococcus lactis. Preferably an enzyme of Escherichia Coli is used.


The peptide deformylases according to the invention require a bivalent metal ion whereby the metal is chosen from the groups 5–11 of the periodic system (New IUPAC version; see Handbook of Chemistry and Physics 70th edition, CRC Press, 1989–1990, inner page of cover), as a cofactor. Preferably the metal is chosen from the group of V, Cr, Fe, Ni, Mn, Co, Cu, Pd and Pt, in particular from the group of Fe, Ni, Mn and Co.


Preferably the amount of the bivalent metal ions should be about equivalent to the number of moles of enzyme. Suitably the molar ratio between these bivalent metal ions and the number of PDF molecules is in the range of 0.6 to 1.4, preferably of 0.8 to 1.2, and most preferred the amount of bivalent metal ions is equimolar to the enzyme.


Exchange of the bivalent metal ions in the PDF's in order to obtain PDF enzymes with a co-factor as necessary for the present invention can be done by the various methods as described in Groche et al., Biochem. Biophys. Res. Comm., 246, 342–346, (1998). These methods include simple metal displacement by incubation of the native enzyme in an excess of the desired bivalent metal ion, if necessary preceeded by the preparation of the apoenzyme via treatment of the native enzyme with a metal chelation compound. Furthermore, the desired bivalent metal ion can already be introduced in (at least part of the enzyme molecules) by using a bacterial growth medium with an enhanced ratio of the desired bivalent metal ion over Fe2+.


In addition measures may be taken in order to enhance the stability of the enzyme, for instance the addition of stabilisation agents, for instance catalase, tris-(2-carboxyethyl)phosphine, glucose oxidase, or combinations thereof; or enlarging the concentration of the PDF, for instance to a PDF concentration of at least 0.1 mg of PDF per ml, more preferably of least 1.0 mg/ml. The upper limit of the concentration of PDF is not critical if practical concentrations are being used. The use of stabilisation measures is especially preferred when an easily oxidisable metal ion, e.g. Fe++ is present as a cofactor or an easily oxidisable substrate. If not, for instance in case Ni++ is present as a cofactor the addition of a stabilisation agent appeared to be superfluous, as the enzyme turned out to be very stable even without stabilisation agent.


The enzymes applied in the process according to the invention may be purified enzymes, a crude enzyme solution, microbial cells exhibiting the required activity, a homogenate of cells or permeabilized cells. If required, the enzyme may be applied in an immobilized state or in a chemically modified form to ensure a good stability, reactivity and enantioselectivity of the enzymes under the conditions utilized.


Alternatively, genetically engineered mutants of PDF's may be used which have for instance enhanced activity or enantioselectivity in the (de)formylation reaction. These mutants can be generated by a number of different approaches; for instance, by site-directed mutagenesis, site-specific random mutagenesis, regio-specific random mutagenesis, and completely random mutagenesis; the latter form of mutagenesis is better known as directed evolution. General applicable methods to perform these different protein engineering approaches are well known to the skilled man. If a random approach will be applied, the mutagenesis cycle will need to be followed by selection of resistent and active mutant(s), thereby leading to the identification of suitable mutants. To obtain PDF mutants also a combination of different protein engineering approaches and/or several rounds of random mutagenesis may be used.


The reaction conditions for the enzymatic deformylation according to the invention are not very critical and may depend on the substrate used. Any suitable solvent system which is inert towards the PDF may be applied; such solvents include aqueous systems (solutions or slurries) or aqueous systems also containing a water-miscible organic solvent which is inert under the reaction conditions. Aqueous systems, however, are preferred. Also the concentration of the N-formyl compound is not critical, and may be for instance in the range of about 0.1 to 1000 mM. It is not necessary that all of the N-formyl compound is dissolved; part of it may be present as a slurry. The concentration of the PDF likewise is not very critical, and usually will be at 0.001 to 100% by weight of the formyl compound, e.g. at about 0.2 mM of PDF. The pH for the reaction preferably is chosen in the range of 4.0 to 11.0, more preferably of 5.0 to 10.0. The temperature is not very critical, and suitably will be in the range of 10 to 50° C., e.g. at about 37° C., but for thermostable PDF enzymes higher temperatures may be applied.


In those cases wherein the absolute configuration of the (de)formylated enantiomer was determined, it appeared that the S-enantiomer was (de)formylated more rapidly than the R-enantiomer. The optical purity is given by the enantiomeric excess (ee), the enantioselectivity of the enzyme is represented by E, and calculated as kf/ks wherein kf is defined as the rate of (de)formylation of the most rapidly (de)formylated enantiomer and ks is defined as the rate of (de)formylation of the least rapidly (de)formylated enantiomer.


Optionally a salt promoting hydrophobic interactions is added to the reaction mixture, for instance a sulphate, phosphate, sulphite or acetate of ammonium, Rb, K, Na, Cs or Li. Most preferably ammonium sulphate or lithium sulphate is used.


The invention will further be elucidated by the following examples, without being limited thereto.


Abbreviations:




  • TB medium: 12 g/l of Bacto-Tryptone, Difco; 24 g/l of yeast extract, Difco; 4 g/l of glycerole; 2.3 g/l of KH2PO4; 12.5 g/l of K2HPO4);

  • Hepes: N-2-hydroxyethylpiperazine-N′-2-ethane sulphuric acid;

  • AEBSF: 2-aminoethyl-p-benzene sulphonyl fluoride;

  • TCEP: tris-(2-carboxyethyl)-phosphine.

  • MOPS: 3-(N-morpholino)propane sulphonic acid

  • MES: 2-(N-morpholino)ethane sulphonic acid








EXAMPLES 1–15
Comparative Experiments A and B

Isolation of PDF(Fe)


For a detailed discussion of the methods used reference is made to Groche et al., BBRC 246, 342–346 (1998).


PDF(Fe) was isolated from overproducing E. coli cells grown at 30° C. in 1.6 l TB medium for 14–16 h. About 13 g (wet weight) cell paste were suspended in 26 ml buffer (20 mM Hepes/KOH, 100 mM KF, pH 7.7 supplemented with 10 μg/ml catalase from bovine liver (Boehringer Mannheim) and 1 mM AEBSF, disintegrated by sonication (Branson B12, 20 min) at 0° C. and centrifuged at 200.000 g for 1 h. The clear supernatant (1.3 g of protein; according to biurete reaction) was mixed with 1.3 ml 10% (w/v) Polymin G-35 (BASF) adjusted to pH 7.7 and centrifuged at 40.000 g for 10 min. The supernatant was applied to a 20 ml Met-Lys-Sepharose column that had been equilibrated with 20 mM Hepes/KOH, 100 mM KF, 0.2 mM TCEP, pH 7.7. After washing with 120 ml of 20 mM Hepes/KOH, 100 mM KF, 0.2 mM TCEP, pH 7.7, PDF(Fe) was eluted with 150 ml 20 mM Hepes/KOH, 100 mM KCl, 0.2 mM TCEP, pH 7.7. The protein containing fractions were concentrated by ultrafiltration using an Amicon PM10 membrane (yield: 140 mg protein, 1400 U/mg; determined according to Groche et al.). After adjustment of the TCEP concentration to 1 mM and protein concentration to 40 mg/ml, the PDF(Fe) stock solution (40 mg/ml=2 mM) was stored frozen at −60° C.


After thawing, the PDF(Fe) stock solution could be used directly in the deformylation experiments described below. If however solutions with lower PDF(Fe) concentrations were required for these deformylation experiments, the PDF stock solution was diluted further in 20 mM Hepes/KOH, pH 7.7, 100 mM KCl, 1 mg/ml bovine serum albumin, 10 μg/ml catalase solution.


HPLC-analysis


In all cases HPLC conditions had to be developed in which the two deformylated isomers were separated from each other and from the formylated isomers. To this end two different techniques were applied that is method 1 and method 2, as described below.


From the quantities of deformylated isomers in the samples after various reaction times, both the initial deformylation rate constant (kf and ks in M−1 s−1 could be calculated for both enantiomers, as well as the respective ee values. The enantioselectivity of the enzyme (E value) was calculated by taking the ratio of kf/ks and is given for all Examples in table 1, as well as the maximum ee value (eemax) observed during the experiments.


Method 1 (Without Derivatization)


A Crownpak CR(+) column (4×150 mm) was used. Samples (5 μl) withdrawn from the deformylation mixture were mixed with 95 μl aqueous HClO4 (10 mM) to inactivate PDF(Fe). Following a brief centrifugation, 20 μl of the supernatant were applied to the Crownpak CR(+) column. For specific chromatographic conditions and retention times see table 2.


Method 2 (Precolumn Derivatization with o-phthaldialdehyde (OPA) and N-acetyl-L-cysteine (NAC).


Samples (25 μl) withdrawn from the deformylation mixture were mixed with 25 μl aqueous HClO4 (100 mM) to inactivate PDF(Fe). Following a brief centrifugation, 40 μl of the supernatant were added to 80 μl 1 M aqueous H3BO3/NaOH pH 9.4, subsequently 20 μl OPA reagent (consisting of OPA in H2O/CH3OH 1:1 v/v with a concentration as indicated in table 3) and 20 μl NAC reagent (consisting of NAC in H2O/CH3OH 1:1 v/v with a concentration as indicated in table 3) was added. After the time indicated in table 3 derivatization was terminated by addition of 80 μl (250 mM) aqueous H3PO4, and 20 μl of the solution were instantaneously applied to a Nucleosil 120-5 C18 (250×4 mm) column. Temperature was always ambient and detection was spectrophotometric using a wavelength of 257 nm and/or 340 nm. The used eluent was a mixture of aqueous 0.05 M H3PO4 brought at pH 7.0 with 1 M NaOH, and a percentage of acetonitrile as indicated in table 3.


For derivatization of valine aminonitrile borate buffer was adjusted to pH 11 and addition of NAC reagent was done 10 min after OPA reagent had been added.


Concentration of H3PO4 used for termination was 500 mM. Derivatization and separation conditions as well as the observed retention times for the deformylated compounds analyzed are compiled in table 3.


Examples 1–12 and comparative experiments A and B were executed according to the procedures A, B, or C as given below as indicated in table 1. The results of the examples and comparative experiments are summarized in table 1 and the corresponding HPLC conditions in tables 2 and 3.


Method A


Deformylation in the Presence of Li2SO4 at pH 7.2


Deformylation reactions were performed in 1.5 ml Eppendorf reaction test tubes. The reaction mixture with a total volume of 200 μl contained 100 mM aqueous MOPS/NaOH, 2 M Li2SO4 buffer pH 7.2, and the concentration of formylated compound as indicated in table 1. After thermal equilibration to 37° C. the deformylation reaction was started by the addition of the concentration of PDF as indicated in table 1. At various reaction times samples of the reaction mixture were withdrawn in which the reaction was stopped by addition of HClO4.


Method B


Deformylation in the Absence of Li2SO4 at pH 7.2


Reactions were performed as described in Method A with the exception that 100 mM aqueous MOPS/NaOH, 250 mM NaCl, 0.1 mg/ml catalase buffer pH 7.2 was used in stead of 100 mM aqueous MOPS/NaOH, 2 M Li2SO4 buffer pH 7.2.


Method C


Deformylation in the Absence of Li2SO4 at pH 6.2


Reactions were performed as described in Method A with the exception that 100 mM aqueous MES/NaOH buffer pH 6.2 was used in stead of 100 mM MOPS/NaOH, 2 M Li2SO4 buffer pH 7.2.









TABLE 1







Results of deformylation experiments


















Type of

[Compound]
[PDF]
ks
kf

eemax


Ex.
Compound
compound
Method
(mM)
(μM)
(M−1s−1)
(M−1s−1)
E
(%)



















1
N-formyl-phenylglycine
α-H-amino acid
B
10
200
0.0047
10.6
2255
99.6


2
N-formyl-3-amino-3-phenyl-
β-H-amino acid
B
10
10
<0.004
7.1
>1775
100



propionic acid


3
N-formyl-phenylglycine
α-H-amino acid
B
10
5.2
0.09
227
2522
99.7



amide
amide


4
N-formyl-tert-leucine
α-H-amino acid
A
4.8
200
0.0005
0.15
300
100



amide
amide


5
N-formyl-α-methyl-
α-alkyl-amino
A
10
200
0.0005
0.045
90
100



phenylglycine amide
acid amide


6
N-formyl-phenylglycinol
β-amino
B
10
200
0.029
0.69
23.8
90.5




alcohol


7
N-formyl-phenylglycinol
β-amino
A
10
200
0.34
6.3
18.5
93.3




alcohol


8
N-formyl-alaninol
β-amino
A
10
200
0.018
0.22
12
85.6




alcohol


9
N-formyl-phenylalanine
α-aminonitrile
C
7.5
20
1
880
880
98.8



aminonitrile


10
N-formyl-valine
α-aminonitrile
A
10
50
0.62
29.7
47.9
95.5



aminonitrile


11
N-formyl-m-methoxy-
α-aminonitrile
B
7.2
2.5
2
1370
685
99.0



phenylalanine aminonitrile


12
N-formyl-1-(1-naphthyl)-
amine
A
0.42
200
0.03
0.45
15
90



ethylamine


A
N-acetyl-phenylglycine
α-H-amino acid
A
10
10
<0.001
<0.001





amide
amide


B
N-formyl-proline
α-H-imino acid
A
10
200
<0.004
<0.004


















TABLE 2







Analytical conditions and retention times analyzed according to method 1









retention time (min)


















flow rate
T
Detection


formyl-


Ex.
Compound
Eluent
(ml/min)
(° C.)
(nm)
Amine
Amine
compound


















1
N-formyl-phenylglycine
10 mM aq. HClO4
1.0
40
210
 2.1(D)
 3.8(L)
9.6


2
N-formyl-3-amino-3-
85% 100 mM aq. HClO4/15%
0.7
5
210
23.7
26.7
11.4



phenyl-propionic acid
CH3OH


3
N-formyl-phenylglycine amide
10 mM aq. HClO4
0.8
22
210
 3.2(D)
12.6(L)
6.3


6/7
N-formyl-phenylglycinol
95% 10 mM aq. HClO4/5%
0.8
5
210
 4.8(L)
 5.7(D)
10.0




CH3OH


9
N-formyl-phenylalanine
90% 10 mM aq. HClO4/10%
0.8
5
210
11.8
15.1
28.6



aminonitrile
CH3OH


11
N-formyl-m-methoxy-
90% 10 mM aq. HClO4/10%
0.8
5
210
23.8
30.7
52.0



phenylalanine aminontrile
CH3OH


12
N-formyl-1-(1-naphthyl)-
85% 10 mM aq. HClO4/15%
1.0
40
210
26.5(S)
31.2(R)
73.5



ethylamine
CH3OH


A
N-acetylphenylglycine amide
10 mM aq. HClO4
0.8
22
210
 3.2 (D)
12.6 (L)
6.9


B
N-formyl-proline
100 mM aq. HClO4
0.4
5
200
 3.8
 3.8
5.7
















TABLE 3







Analytical conditions and retention times analyzed according to method 2
















OPA
NAC
Time
%
Retention
Amine


Ex.
Compound
(mg/ml)
(mg/ml)
(min.
CH3CN
Time (min.)
Amineformyl

















2
N-formyl-3-amino-3-phenyl
4
4
30
15
19.7
23.3



propionic acid


4
N-formyl-tert-leucine amide
8
8
10
22.5
14.9 (D)
17.4 (L)


5
N-formyl-α-methyl-
16
16
30
20
24.4
26.3



phenylglycine amide


8
N-formyl-alaninol
4
4
5
15
16.9(L)
18.8(D)


10
N-formyl-valine aminonitrile
16
4
5
20
 8.6 (L)
10.2 (D)








Claims
  • 1. A process for the preparation of a compound with enhanced optical purity which comprises contacting a mixture of the enantiomers of a chiral compound of formula 1
  • 2. The process of claim 1 wherein the formylating agent is formic acid, a formic acid amide or a formic acid ester.
  • 3. The process of claim 1, wherein the peptide deformylase is of the class EC 3.5.2.27 or EC 3.5.1.31.
  • 4. The process of claim 1, wherein the peptide deformylase contains the sequences (I) HEXXH, (ii) EGCLS and (iii) GXGXAAXQ.
  • 5. The process of claim 1, wherein the peptide deformylase is obtainable from Escherichia coli.
  • 6. The process of claim 1, wherein the bivalent metal is Fe, Ni, Mn or Co.
  • 7. The process of claim 6, wherein the bivalent metal is Ni.
  • 8. The process of claim 6 wherein the bivalent metal is Fe.
  • 9. The process of claim 1, which further comprises adding a stabilisation agent.
  • 10. The process of claim 8 wherein the stabilisation agent is catalase.
Priority Claims (1)
Number Date Country Kind
98204371 Dec 1998 EP regional
CROSS-REFERENCE TO RELATED APPLICATIONS

This Application is a divisional of U.S. Ser. No. 09/869,088 filed 19 Jun. 2001 and now U.S. Pat. No. 7,018,817, which is the national phase of PCT application PCT/NL99/00783, filed 17 Dec. 1999, which claims priority from European application 98/204371.3 filed 22 Dec. 1998. The contents of these applications are incorporated herein by reference.

US Referenced Citations (2)
Number Name Date Kind
4745067 Umezawa et al. May 1988 A
6617127 Quaedflieg et al. Sep 2003 B1
Foreign Referenced Citations (1)
Number Date Country
WO-9850575 Nov 1998 WO
Related Publications (1)
Number Date Country
20060127997 A1 Jun 2006 US
Divisions (1)
Number Date Country
Parent 09869088 US
Child 11350647 US