Biodegradation of Aliphatic-Aromatic Copolyesters by Thermomonospora fusca and Other Thermophilic Compost Isolates

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Kleeberg, I.
	Articles by Deckwer, W.-D.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Kleeberg, I.
	Articles by Deckwer, W.-D.


Agricola

	Articles by Kleeberg, I.
	Articles by Deckwer, W.-D.

Previous Article | Next Article

Appl Environ Microbiol, May 1998, p. 1731-1735, Vol. 64, No. 5
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Biodegradation of Aliphatic-Aromatic Copolyesters by Thermomonospora fusca and Other Thermophilic Compost Isolates

Ilona Kleeberg,¹ Claudia Hetz,¹ Reiner Michael Kroppenstedt,² Rolf-Joachim Müller,¹^,^* and Wolf-Dieter Deckwer¹

Gesellschaft für Biotechnologische Forschung mbH¹ and Deutsche Sammlung für Mikroorganismen und Zellkulturen,² D-38124 Braunschweig, Germany

Received 6 October 1997/Accepted 6 March 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results & Discussion References

Random aliphatic-aromatic copolyesters synthesized from 1,4-butanediol, adipic acid, and terephthalic acid (BTA) have excellentthermal and mechanical properties and are biodegradable by mixedcultures (e.g., in compost). Over 20 BTA-degrading strains wereisolated by using compost as a microbial source. Among these microorganisms,thermophilic actinomycetes obviously play an outstanding roleand appear to dominate the initial degradation step. Two actinomycetestrains exhibited about 20-fold higher BTA degradation rates thanusually observed in a common compost test. These isolates wereidentified as Thermomonospora fusca strains. They appeared tobe particularly suitable for establishment of rapid degradationtests and were used in comparative studies on the biodegradationof various polyesters.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results & Discussion References

Polymers designed to undergo controlled biological degradation are increasingly discussed as a favorable contribution to thesolution of problems arising from plastic waste disposal, e.g.,by recycling or land filling. The environmental safety of thesenovel materials has to be proven carefully (32). A number ofstandardized test methods using mixed cultures for evaluationof the biodegradability and compostability of plastics have beenestablished recently (1, 5, 25, 30). However, for investigationsof the degradation mechanism, it is advantageous to isolate individualstrains which are able to degrade well-defined polymers.

For some polymers, including isoprene rubbers (7, 16, 34), polyvinyl alcohol (29), cellulose acetate (23), poly( $varepsilon$ -polycaprolactone)(24), and bacterial polyhydroxyalkanoates (6), a number ofdegrading microorganisms are described in the literature.

Recently, it has been shown that copolyesters containing adipic acid and terephthalic acid as aromatic acid components arealso attacked by microorganisms (35). This group of copolyestersappears to be very promising with regard to widespread commercialapplications (38). Studies have been performed with the particulargoal of detecting the fate of the aromatic constituents and provingtheir biodegradation (36, 37).

However, in all previous investigations, inocula of undefined mixed cultures were used. Therefore, this study concentratedon the isolation of individual strains which are able to degraderandom aliphatic-aromatic copolyesters. As composting is the mostpromising method of treating such biodegradable plastics, themicrobial isolates were obtained from compost material. The isolatesare appropriate candidates for use in the study of the mechanismof copolyester degradation and the establishment of improved andrapid test methods for evaluation of biodegradability.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results & Discussion References

Polymers. A copolyester made of 1,4-butanediol, terephthalic acid, and adipic acid (Fig. 1) was used to isolate degradative microorganisms.The origins, compositions, melting temperatures, and average molarmasses of all of the polymers tested in the biodegradation studiesare listed in Table 1. Polymer films 100 µm thick and 25 mm indiameter were prepared as described by Witt et al. (35). Thefilms were washed in a 70% (vol/vol) ethanol solution for 30 min,dried at room temperature under a vacuum, and weighed to an accuracyof ±0.2 mg. For sterilization, polymer films were irradiated undera UV lamp (UVC 30; Hereaus, Hannover, Germany; 254 nm, 6 W/cm² at a distance of 20 cm) at a lamp-to-film distance of 15 cm andan irradiation area of 38 by 18 cm for 15 min of exposure perside.

View larger version (10K):
[in this window]
[in a new window]

FIG. 1. Formula of the aliphatic-aromatic copolyester BTA 40:60 used for the screening of microorganisms with regard to their degradation abilities. The copolyester consists of 1,4-butanediol, terephthalic acid, and adipic acid.

View this table:
[in this window]
[in a new window]

TABLE 1. Compositions, melting temperatures, and average molar masses of tested polymers

Source of organisms. Aerobic microorganisms were isolated from samples of approximately 6-month-old mature compost made from green waste (CompostPlant Watenbüttel, Watenbüttel, Germany).

Media and buffer. The compositions of the media used are listed in Table 2 (3a, 4, 14). To retard drying of the agar media at high temperatures,petri dishes were incubated in sealed polyethylene bags (18).For preparation of suspensions and dilutions, a phosphate buffer(0.05 M Na₂HPO₄, 0.03 M KH₂PO₄, pH 7.0) was used.

View this table:
[in this window]
[in a new window]

TABLE 2. Cultivation media

Isolation of BTA-degrading microorganisms. An at least four-step procedure turned out to be the appropriate strategy for the isolation of BTA-degrading strains. Mixedpopulations were used as inocula. These were taken by either (i)scraping off and dissolving (2 ml of phosphate buffer) preadaptedbiofilms grown on BTA films which were incubated in compost reactorsas described by Witt et al. (35) or (ii) dissolving 10 g ofmature compost or compost harvested from reactors in 90 ml ofphosphate buffer.

For enrichment of BTA-degrading microorganisms on agar plates, BTA films were inoculated with 100 µl of the inocula mentionedabove. Different mineral salt and compost extract agar plateswere used as enrichment media (Table 2). The enrichment cultureswere incubated at 20, 40, and 55°C and examined daily for growthof colonies and visible disintegration of the polymer films.

For isolation, colonies were picked up from partly disintegrated areas of films and cultured on various complex agar media(Table 2) by using different inoculation techniques to providefavorable growth conditions for a wide range of microorganisms.

We could not produce homogeneous opaque top layer agar plates with granules of BTA (aggregation of particles due to the hydrophobicsurfaces). Thus, direct selection of degrading microorganismsby a clear-zone method (2) was not possible. Because of theseproblems, the abilities of all isolates to degrade the copolyesterBTA 40:60 had to be tested in a separate step.

The degradation test was carried out with polymer films on three mineral salt media and one compost extract medium (Table2) on agar plates inoculated with actinospore or bacterial suspensions( $approx$ 10⁷ microorganisms/ml) at the optimal growth temperature of the isolates.As an indicator for degradation, the weight loss of the polymerfilms was determined after 14 days of incubation. The resultswere compared with those obtained with noninoculated films (noninoculatedcontrols) incubated in the respective media. The noninoculatedcontrols showed no weight loss.

Cultivation and preservation of isolated strains. The isolates were maintained on agar plates of complex media at temperatures satisfying the individual requirements for optimalgrowth (Table 3). Bacterial strains were preserved in 50% (vol/vol)glycerol at $-$ 20°C. For recultivation, 1 loopful of each glycerolsuspension was streaked onto an NB agar plate (Table 2). After48 h of incubation, single colonies were picked and suspendedin 1 ml of phosphate buffer. These bacterial suspensions servedas the inoculum for degradation tests.

View this table:
[in this window]
[in a new window]

TABLE 3. Incubation temperatures and media for cultivation and testing of BTA-degrading isolates

For preservation of the isolated actinomycete strains, spores from well-sporulating actinomycete cultures were suspended indistilled water and kept at 4°C in screw-cap tubes. Spore suspensionsroutinely served as an inoculum source for degradation tests.

Determination of the optimum growth temperatures of the individual strains was carried out on sections of agar plates inoculatedwith 1 loopful of an actinospore or bacterial suspension and incubatedat temperatures of 20 to 70°C. Aerial mycelium formation and/orcolony growth was visually observed after 1 and 2 weeks. All furthertests were carried out at the respective optimum temperature.

For chemotaxonomic analysis, actinomycete cells were grown in TSB shake flask cultures, harvested by centrifugation (20 min,7,800 × g, 4°C), washed twice in phosphate buffer, and freeze-driedto provide cell preparations (exception: for analysis of fattyacids, wet cells were used).

Taxonomic studies. For 16S ribosomal DNA (rDNA) sequencing, the genomic DNAs of K13g and K7a-3 were extracted and the 16S rRNA gene was amplifiedby PCR as described previously (27). Purified PCR products weredirectly sequenced by using the Taq Dye Deoxy Terminator CycleSequencing Kit (Applied Biosystems, Inc., Foster City, Calif.).Sequences were manually aligned with representatives of relatedsporoactinomycete taxa by using the ae2 editor available fromthe Ribosomal Database Project (17). The diagnostic regionsof the 16S rDNA sequences were compared with those of the Thermomonosporatype strains (28). Direct sequence similarities were calculatedwithin the ae2 editor.

Analysis of cell wall amino acids and sugars. Amino acid and sugar analysis of the whole-cell hydrolysate was done as described by Staneck and Roberts (31).

Extraction and analysis of isoprenoid quinones and polar lipids. Isoprenoid quinones and polar lipids were extracted and purified by the small-scale integrated procedure of Minnikin et al.(21). The dried preparations of the quinone extracts were dissolvedin 200 µl of isopropanol, and 1- to 10-µl amounts were separatedby high-pressure liquid chromatography. The menaquinones wereseparated by high-pressure liquid chromatography on LichrosorbRP-18 at 40°C using acetonitrile-isopropanol (65:35, vol/vol)as the solvent (10, 11). Polar lipid extracts were separatedby two-dimensional thin-layer chromatography and identified bytheir R_f values and their reaction with diagnostic spray reagents(21).

Extraction and analysis of fatty acids. Fatty acid methyl esters were obtained from 40 mg of wet cells by saponification, methylation, and extraction by using minormodifications (15) of the method of Miller (20). The fattyacid methyl ester mixtures were separated by using a 5898A MicrobialIdentification System (Microbial ID, Newark, Del.). Peaks wereautomatically integrated and fatty acids were identified by theMicrobial Identification System Standard Software (Microbial ID).

	RESULTS AND DISCUSSION

Top Abstract Introduction Materials & Methods Results & Discussion References

Screening and isolation of microorganisms. Although it was expected that BTA-degrading microorganisms would be enriched in biofilms grown on BTA films during composting,there was no significant difference in the number of BTA-degradingstrains isolated from compost eluates or preadapted biofilms.

Table 3 gives the isolates, their optimal growth temperatures, and the media on which the isolates revealed the highest BTAdegradation. As expected, different isolates showed maximal activitieson different media, none of which generally appeared to be thebest. Further degradation tests with individual strains were thencarried out with the appropriate media. We obtained the best degradationresults with temperatures higher than 40°C; thus, we focused predominantlyon thermophilic microorganisms.

It must be admitted that weight loss measurements only indicate disintegration of the polymer films likely caused by cleavageof the polymer chains. Complete metabolism of the polymer materialhas to be investigated in additional tests. However, for polyesters,the first step in attacking the polymer chain is often the stepwhich determines the degradability of such materials.

Table 4 gives an overview of the number of isolated bacteria, actinomycetes, and fungi and their abilities to degrade thealiphatic-aromatic copolyester BTA 40:60. A total of 61 strainsof thermophilic microorganisms were isolated from 13 differentcompost samples.

View this table:
[in this window]
[in a new window]

TABLE 4. Numbers of microorganisms isolated and their abilities to degrade the aliphatic-aromatic copolyester BTA 40:60^a

Among 30 bacterial isolates, which were all aerobically growing rods mainly with endospore formation, only five strains wereable to disintegrate BTA 40:60. Three of those strains exhibitedonly weak degradation activities (weight losses of 0.06 to 0.15mg/week · cm²), just above the experimental error of the detection method used.Most fungi grow at temperatures of less than 50°C. This mightbe the reason why we isolated just two strains of fungi. Bothstrains were unable to disintegrate the copolyester BTA 40:60.

Within the group of thermophilic actinomycetes, only 4 of 29 isolates did not show significant degradation activities. Twoof the most active actinomycetes, isolates K13g and K7a-3, wereidentified taxonomically and used for further investigations.They degraded films 100 µm thick up to 90% within 7 days.

More than 20 different microorganisms isolated from compost were able to depolymerize the synthetic polyester BTA 40:60. Probablydue to the use of compost as the source of microorganisms, mostisolates were thermophilic microorganisms. Especially, thermophilicactinomycetes play an outstanding role in degrading the BTA copolyesterwith regard to both the number of microorganisms isolated andtheir degradation rates. Actinomycetes are known to be involvedin the degradation of several natural polymers, like chitin, celluloses,starch, agar, and lignocelluloses (3, 9, 18, 19). However,the role of this group of microorganisms in degrading syntheticpolymers is rarely described in the literature (26).

Identification of selected strains. The phenotypic and chemotaxonomic properties of strains K13g and K7a-3 are consistent with their classification in the genusThermomonospora (13). The strains showed generation of a whiteaerial mycelium and individual spores which were formed in clusterson the tip of a short sporophore. Both strains have the same chemotaxonomiccharacteristics which are consistent with members of the Thermomonosporafusca taxon (13). The whole-cell hydrolysates of strain K13gand K7a-3 contained glucose and ribose as major sugars. Mesodiaminopimelicacid was the only diamino acid found in the cell walls. The polarlipids were composed of diphosphatidylglycerol, phosphatidylglycerol,phosphatidylinositol, phosphatidylethanolamine, methylphosphatidylethanolamine,and some unspecified glycolipids. The fatty acid pattern of thestrains contained mainly iso- and anteiso-branched fatty acids.Small amounts of 10-methyl branched and unbranched fatty acidswere also found.

MK-11(H₄), MK-11(H₆), MK-12(H₄), and MK-12(H₆) were the predominant menaquinones of both strains. The combination of chemicalmarkers found in K13g and K7a-3 is unique to the strains of T.fusca. Therefore, K13g and K7a-3 could be classified as T. fuscaby chemotaxonomy. This was confirmed by the analysis of 16S rDNAsequences of both isolates, which showed that isolates K7a-3 andK13g belong to the family Thermomonosporaceae. The greatest similaritieswere found between the isolates and T. fusca DSM 43792^T (K7a-3, 100%; K13g, 99.8%). Obviously, these two actinomyceteisolates are representatives of this species.

BTA film degradation on agar plates by T. fusca K13g. With regard to the application of isolated strains as test organisms in improved degradation tests, the time course of thedegradation of BTA films on agar plates by T. fusca K13g was investigated.Usually, enzymatic degradation of plastics is a surface erosionprocess, because enzymes are not able to penetrate the bulk polymer.Thus, the rate of weight loss can be directly used to measurethe enzymatic cleavage of the polymer chains.

In Fig. 2, the weight loss of BTA films inoculated with a spore suspension of the actinomycete T. fusca K13g is plotted againstthe degradation time. A short period of only 7 days was sufficientto completely disintegrate the BTA films on the agar plates, resultingin a weight loss curve often observed for biological transformations.During a lag phase of 1 day, actinospores germinated; this wasfollowed by a period of 3 days with constant weight loss of theexposed films. As the films started to fall into fragments, thedegradation rate decreased gradually, and after 1 week, the BTAmaterial disappeared totally. Although this high degree of degradationand the fact that the curve was obtained from films in paralleltests stopped at different times after incubation, the reproducibilityof this experiment was very good.

View larger version (14K):
[in this window]
[in a new window]

FIG. 2. Degradation of the aliphatic-aromatic copolyester BTA 40:60 on agar plates by the actinomycete T. fusca K13g. The test was carried out on MSV agar over a period of 13 days at 55°C with triplicate samples. From day 6 on, error bars are not shown because polymer films (diameter, 2.5 cm; thickness, 90 µm; initial weight, 46 mg; degradation area, 4.91 cm²) disappeared according to their initial weights (light films first) and error bars would represent the differences between the initial weights from that day on.

By calculating specific degradation rates from the linear part of the degradation curves in combination with the surface areaof the films which could be attacked by the organisms, differentexperiments can be compared with regard to the degradation potentialof the organisms involved.

Typical degradation rates of about 1 mg/week · cm² were obtained for BTA 40:60 films in a compost simulation test. Significantlyhigher degradation rates of up to 2.3 mg/week · cm² were found with preadapted mixed cultures from compost in anagar plate test. However, the increase in the degradation ratefrom compost to the preadapted mixed culture is not only relatedto the higher degradation potential of the organisms but alsoinfluenced by the optimized degradation conditions in the laboratoryagar plate test. Remarkable degradation rates as high as 20 mg/week· cm² could be obtained with the actinomycete T. fusca K13g under definedlaboratory conditions, which are about 10-fold higher than thoseachieved for the copolyester films incubated with adapted mixedcultures.

Compared to the fast degradation of T. fusca K13g, the degradation rate of bacterial strains K1a-1 and K1a-2 was quite slow.A continuous degradation of BTA films of only 0.1 mg/week · cm² within a test period of 6 weeks was observed.

The fast degradation of the BTA copolyester, in combination with the good reproducibility of the degradation rates in agarplate tests, predestine the actinomycete T. fusca K13g for usein rapid test methods and fundamental investigations of the degradationmechanism of the BTA copolyester and other polyesters as well.

Degradation of different kinds of polymers by two actinomycete isolates. The aromatic-aliphatic copolyester BTA 40:60 used for the screening is a biodegradable polymer of high commercial interestbut does not occur in nature. Thus, to determine the substratespecificity of the isolated microorganisms, we tested the degradationof other polyesters and one polyester amide (Fig. 3) by T. fuscaK13g and K7a-3. The two strains exhibited similarly high BTA 40:60degradation abilities.

View larger version (29K):
[in this window]
[in a new window]

FIG. 3. Degradation of different polyesters and the polyester amide Bayer Tir 1874 on agar plates by T. fusca K7a-3 and K13g. Polymer films (diameter, 2.5 cm; degradation area, 4.91 cm²) were incubated at 55°C for 2 weeks on MSV agar. A second test series gave reproducible results. Each series was carried out with triplicate samples. The degradation rate was calculated with data from the linear part of the degradation curve.

In all cases, the degradation rates obtained with strain K7a-3 were somewhat lower than those of strain K13g. Of the polyester-basedmaterials tested, the aliphatic-aromatic copolyester BTA 40:60exhibited the highest degradation rate, while pure aliphatic materialslike Bionolle, Bayer Tir 1874, or even the bacterial polyesterpoly( $beta$ -hydroxybutyrate) (PHB) were degraded much more slowly byboth strains. This is surprising in that these polyesters areregarded to be easily biodegradable. Even a copolyester containing60 mol% terephthalic acid disintegrates almost twice as fast asthe natural material PHB. Polyesters with such a large aromaticcompound fraction have been shown to degrade only very slowlyin composting tests (35). The degradation behavior of SP313is also unexpected. This aliphatic polyester with a long diacidcomponent is not easily degraded in soil burial tests or in enzymaticdegradation tests with lipases (22).

It can be anticipated that both thermophilic actinomycetes and their enzymatic systems prefer hydrophobic surfaces such asthose offered by BTA copolyesters or the aliphatic polyester SP313.It will be challenging and illuminating to isolate and characterizethe enzymatic system responsible for polymer chain cleavage andto compare its components with other polyester-degrading enzymeslike lipases or PHB depolymerases (8, 33).

Despite the rapid depolymerization of the BTA copolyester, only poor growth of the actinomycetes could be observed on mineralsalt agar with a polymer as the sole carbon source. This suggeststhat the actinomycetes are not able to completely metabolize theoligomers and monomers derived from the depolymerization of thepolyester. As BTA copolyesters are abiotic synthetic materials,it is not likely that microorganisms have been specialized tothis kind of carbon source. However, they are adapted to the useof other, similar polyester structures containing aromatic componentslike those in cutin or lignocelluloses.

Further investigations are in preparation to clarify the mechanism of BTA copolyester degradation by actinomycetes and toidentify the enzymes involved.

	ACKNOWLEDGMENTS

We thank B. Frerichs, G. Pötter, I. Kramer, and J. Swiderski for their skilled technical assistance.

	FOOTNOTES

^* Corresponding author. Mailing address: Gesellschaft für Biotechnologische Forschung mbH, Mascheroder Weg 1, 38124 Braunschweig,Germany. Phone: 49 531 6181610. Fax: 49 531 6181175. E-mail: rmu{at}gbf.de.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results & Discussion
References

1. American Society for Testing and Materials. 1996. In D 6002-96. Standard guide for assessing the compostability of environmentally degradable plastics. American Society for Testing and Materials, Washington, D.C.

2. Augusta, J., R.-J. Müller, and H. Widdecke. A rapid evaluation plate-test for the biodegradability of plastics. Appl. Microbiol. Biotechnol. 39:673-678.

3. Crawford, D. L., and J. B. Sutherland. 1980. Isolation and characterization of lignocellulose-decomposing actinomycetes, p. 95-101. In T. K. Kirk, T. Higuchi, and H. Chang (ed.), Lignin biodegradation: microbiology, chemistry, and potential applications, vol. II. CRC Press, Inc., Bota Raton, Fla.

3a. Deutsche Sammlung von Mikroorganismen und Zellkulturen. 1993. In DSM 65. DMS-catalogue of strains 1993, fifth ed., p. 357. Deutsche Sammlung von Mikroorganismen und Zellkulturen, Braunschweig, Germany.

4. Deutsches Institut für Normung e.V. 1984. In DIN 53749. Lösungen und Nährmedien für die Prüfung mit Bakterien, p. 3. Beuth Verlag GmbH, Berlin, Germany.

5. Deutsches Institut für Normung e.V. 1997. In DIN 54900-Entwurf. Prüfung der Kompostierbarkeit von polymeren Werkstoffen, p. 1-7. Beuth Verlag GmbH, Berlin, Germany.

6. Doi, Y. 1990. In Microbial polyesters. VCH Publishers Inc., New York, N.Y.

7. Heisey, R. M., and S. Papadatos. 1995. Isolation of microorganisms able to metabolize purified natural rubber. Appl. Environ. Microbiol. 61:3092-3097[Abstract].

8. Jaeger, K.-E., A. Steinbüchel, and D. Jendrossek. 1995. Substrate specificities of bacterial polyhydroxyalkanoate depolymerases and lipases: bacterial lipases hydrolyze poly( $omega$ -hydroxyalkanoates). Appl. Environ. Microbiol. 61:3113-3118[Abstract].

9. Kempf, A., and H. J. Kutzner. 1988. Screening von biopolymerabbauenden Exoenzymen bei thermophilen Actinomyceten, p. 979-989. In VDLUFA-Schriftenreihe 28. Kongressband Teil II, Oldenburg, Germany.

10. Kroppenstedt, R. M., F. Korn-Wendisch, V. J. Fowler, and E. Stackebrandt. 1981. Biochemical and molecular genetic evidence for transfer of Actinoplanes armeniacus into the family Streptomycetaceae. Zentbl. Bakteriol. Hyg. Abt. Orig. C2:254-262.

11. Kroppenstedt, R. M. 1985. Fatty acid and menaquinone analysis of actinomycetes and related organisms, p. 173-199. In M. Goodfellow, and D. E. Minnikin (ed.), Chemical methods in bacterial systematics. Academic Press, Inc., New York, N.Y.

12. Kroppenstedt, R. M. 1992. The genus Nocardiopsis, p. 1139-1156. In A. Balows, H. G. Trüper, M. Dworkin, W. Harder, and K. H. Schleifer (ed.), The prokaryotes, a handbook on the biology of bacteria; ecophysiology, isolation, identification, applications, 2nd ed., vol. II. Springer-Verlag KG, Berlin, Germany.

13. Kroppenstedt, R. M., and M. Goodfellow. 1992. The family Thermomonosporaceae, p. 1085-1114. In A. Balows, H. G. Trüper, M. Dworkin, W. Harder, and K. H. Schleifer (ed.), The prokaryotes, a handbook on the biology of bacteria: ecophysiology, isolation, identification, applications, 2nd ed., vol. II. Springer-Verlaq KG, Berlin, Germany.

14. Küster, E., and S. T. Williams. 1964. Selection of media for isolation of streptomycetes. Nature (London) 202:928-929[Medline].

15. Kuykendall, L. D., M. A. Roy, J. J. O'Neill, and T. E. Devine. 1988. Fatty acids, antibiotic resistance, and deoxyribonucleic acid homology groups of Bradyrhizobium japonicum. Int. J. Syst. Bacteriol. 38:358-361[Abstract/Free Full Text].

16. Linos, A., and A. Steinbüchel. 1996. Investigations on the microbial breakdown of natural and synthetic rubber, p. 211-219. In Proceedings of the 10th International Biodeterioration and Biodegradation Symposium. VCH-Verlag, Weinheim, Germany.

17. Maidak, B. L., N. Larsen, M. J. McCoughey, R. Overbeek, G. J. Olsen, K. Folgel, J. Blandy, and C. R. Woese. 1994. The Ribosomal Database Project. Nucleic Acids Res. 22:3485-3487[Abstract/Free Full Text].

18. McCarthy, A. J., and T. Cross. 1984. A taxonomic study of Thermomonospora and other monosporic actinomycetes. J. Gen. Microbiol. 130:5-25.

19. McCarthy, A. J. 1987. Lignocelllulose-degrading actinomycetes. FEMS Microbiol. Rev. 46:145-163.

20. Miller, L. T. 1982. A single derivatization method for routine analysis of bacterial whole-cell fatty acid methyl esters, including hydroxy acids. J. Clin. Microbiol. 16:584-586[Abstract/Free Full Text].

21. Minnikin, D. E., A. G. O'Donnel, M. Goodfellow, G. Alberton, M. Ethel, A. Scale, and J. H. Parlayed. 1984. An integrated procedure for the extraction of isoprenoid quinones and polar lipids. J. Microbiol. Methods 2:233-241.

22. Müller, R.-J. 1996. Mechanistic studies on the biodegradation of polyesters, p. 211-219. In Proceedings of the 10th International Biodeterioration and Biodegradation Symposium. VCH-Verlag, Weinheim, Germany.

23. Nelson, M., S. P. McCarthy, and R. A. Gross. 1992. Isolation of a Pseudomonas paucimobilis capable of using insoluble cellulose acetate as a sole carbon source. Polym. Mater. Sci. Eng. 67:139-140.

24. Nishida, H., and Y. Tokiwa. 1992. Distribution of poly( $beta$ -hydroxybutyrate) and poly( $varepsilon$ -caprolactone) degrading microorganisms and microbial degradation behaviour on plastic surfaces. Polym. Mater. Sci. Eng. 67:137-138.

25. Pagga, U. Biodegradability and compostability of polymeric materials in the context of the European packaging regulation. In Proceedings of the International Conference on Advanced Materials, in press.

26. Pommer, E. H. 1995. Synthetische organische Materialien, p. 111-150. In H. Brill (ed.), Mikrobielle Materialzerstörung und Materialschutz: Schädigungsmechanismen und Schutzmaßnahmen. Gustav Fischer Verlag, Jena, Germany.

27. Rainey, F. A., M. Dorsch, H. W. Morgan, and E. Stackebrandt. 1992. 16S rDNA analysis of Spirochaeta thermophila: its phylogenetic position and implications for systematics of the order Spirochaetales. Syst. Appl. Microbiol. 15:197-202.

28. Rainey, F. A., N. Ward-Rainey, R. M. Kroppenstedt, and E. Stackebrandt. 1996. The genus Nocardiopsis represents a phylogenetically coherent taxon and a distinct actinomycete lineage: proposal of Nocardiopsaceae fam. nov. Int. J. Syst. Bacteriol. 46:1088-1092[Abstract/Free Full Text].

29. Sakai, K., N. Hamada, and Y. Watanabe. 1986. Degradation mechanism of poly(vinyl alcohol) by successive reactions of secondary alcohol oxidase and $beta$ -diketone hydrolase from Pseudomonas sp. Agric. Biol. Chem. 50:989-996.

30. Sawada, H. ISO standard activities in standardization of biodegradable and/or compostable polymers; development of test methods, definitions. In Proceedings of the International Conference on Advanced Materials, in press.

31. Staneck, J. L., and G. D. Roberts. 1974. Simplified approach to identification of aerobic actinomycetes by thin-layer chromatography. Appl. Microbiol. 28:226-231[Medline].

32. Swift, G. 1992. Biodegradable polymers in the environment: are they really biodegradable? Polym. Mater. Sci. Eng. 66:403-404.

33. Tokiwa, Y., T. Ando, T. Suzuki, and K. Takeda. 1990. Biodegradation of synthetic polymers containing ester bonds. Am. Chem. Soc. Symp. Ser. 433:136-148.

34. Tsuchii, A., and K. Takeda. 1990. Rubber-degrading enzyme from a bacterial culture. Appl. Environ. Microbiol. 56:1-269[Abstract/Free Full Text].

35. Witt, U., R.-J. Müller, and W.-D. Deckwer. 1995. New biodegradable polyester-copolymers from commodity chemicals with favourable use properties. J. Environ. Polym. Degrad. 3:215-223.

36. Witt, U., R.-J. Müller, and W.-D. Deckwer. 1996. Evaluation of the biodegradability of copolyesters containing aromatic compounds by investigations of model oligomers. J. Environ. Polym. Degrad. 4:9-20.

37. Witt, U., R.-J. Müller, and W.-D. Deckwer. 1996. Studies on sequence distribution of aliphatic/aromatic copolyesters by high-resolution ¹³C nuclear magnetic resonance spectroscopy for evaluation of biodegradability. Makromol. Chem. Phys. 197:1525-1535.

38. Witt, U., R.-J. Müller, and W.-D. Deckwer. 1997. Biodegradation behaviour and material properties of aliphatic/aromatic polyesters of commercial importance. J. Environ. Polym. Degrad. 5:81-89.

This article has been cited by other articles:

Akutsu-Shigeno, Y., Teeraphatpornchai, T., Teamtisong, K., Nomura, N., Uchiyama, H., Nakahara, T., Nakajima-Kambe, T. (2003). Cloning and Sequencing of a Poly(DL-Lactic Acid) Depolymerase Gene from Paenibacillus amylolyticus Strain TB-13 and Its Functional Expression in Escherichia coli. Appl. Environ. Microbiol. 69: 2498-2504 [Abstract] [Full Text]
Lyon, P.-F., Beffa, T., Fischer, J. L., Aragno, M. (2000). Xylanase activity and thermostratification during the thermogenic phase of industrial composting in aerated trenches. Waste Manag Res 18: 174-183 [Abstract]

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Kleeberg, I.
	Articles by Deckwer, W.-D.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Kleeberg, I.
	Articles by Deckwer, W.-D.


Agricola

	Articles by Kleeberg, I.
	Articles by Deckwer, W.-D.

1.	American Society for Testing and Materials. 1996. In D 6002-96. Standard guide for assessing the compostability of environmentally degradable plastics. American Society for Testing and Materials, Washington, D.C.
2.	Augusta, J., R.-J. Müller, and H. Widdecke. A rapid evaluation plate-test for the biodegradability of plastics. Appl. Microbiol. Biotechnol. 39:673-678.
3.	Crawford, D. L., and J. B. Sutherland. 1980. Isolation and characterization of lignocellulose-decomposing actinomycetes, p. 95-101. In T. K. Kirk, T. Higuchi, and H. Chang (ed.), Lignin biodegradation: microbiology, chemistry, and potential applications, vol. II. CRC Press, Inc., Bota Raton, Fla.
3a.	Deutsche Sammlung von Mikroorganismen und Zellkulturen. 1993. In DSM 65. DMS-catalogue of strains 1993, fifth ed., p. 357. Deutsche Sammlung von Mikroorganismen und Zellkulturen, Braunschweig, Germany.
4.	Deutsches Institut für Normung e.V. 1984. In DIN 53749. Lösungen und Nährmedien für die Prüfung mit Bakterien, p. 3. Beuth Verlag GmbH, Berlin, Germany.
5.	Deutsches Institut für Normung e.V. 1997. In DIN 54900-Entwurf. Prüfung der Kompostierbarkeit von polymeren Werkstoffen, p. 1-7. Beuth Verlag GmbH, Berlin, Germany.
6.	Doi, Y. 1990. In Microbial polyesters. VCH Publishers Inc., New York, N.Y.
7.	Heisey, R. M., and S. Papadatos. 1995. Isolation of microorganisms able to metabolize purified natural rubber. Appl. Environ. Microbiol. 61:3092-3097[Abstract].
8.	Jaeger, K.-E., A. Steinbüchel, and D. Jendrossek. 1995. Substrate specificities of bacterial polyhydroxyalkanoate depolymerases and lipases: bacterial lipases hydrolyze poly( $omega$ -hydroxyalkanoates). Appl. Environ. Microbiol. 61:3113-3118[Abstract].
9.	Kempf, A., and H. J. Kutzner. 1988. Screening von biopolymerabbauenden Exoenzymen bei thermophilen Actinomyceten, p. 979-989. In VDLUFA-Schriftenreihe 28. Kongressband Teil II, Oldenburg, Germany.
10.	Kroppenstedt, R. M., F. Korn-Wendisch, V. J. Fowler, and E. Stackebrandt. 1981. Biochemical and molecular genetic evidence for transfer of Actinoplanes armeniacus into the family Streptomycetaceae. Zentbl. Bakteriol. Hyg. Abt. Orig. C2:254-262.
11.	Kroppenstedt, R. M. 1985. Fatty acid and menaquinone analysis of actinomycetes and related organisms, p. 173-199. In M. Goodfellow, and D. E. Minnikin (ed.), Chemical methods in bacterial systematics. Academic Press, Inc., New York, N.Y.
12.	Kroppenstedt, R. M. 1992. The genus Nocardiopsis, p. 1139-1156. In A. Balows, H. G. Trüper, M. Dworkin, W. Harder, and K. H. Schleifer (ed.), The prokaryotes, a handbook on the biology of bacteria; ecophysiology, isolation, identification, applications, 2nd ed., vol. II. Springer-Verlag KG, Berlin, Germany.
13.	Kroppenstedt, R. M., and M. Goodfellow. 1992. The family Thermomonosporaceae, p. 1085-1114. In A. Balows, H. G. Trüper, M. Dworkin, W. Harder, and K. H. Schleifer (ed.), The prokaryotes, a handbook on the biology of bacteria: ecophysiology, isolation, identification, applications, 2nd ed., vol. II. Springer-Verlaq KG, Berlin, Germany.
14.	Küster, E., and S. T. Williams. 1964. Selection of media for isolation of streptomycetes. Nature (London) 202:928-929[Medline].
15.	Kuykendall, L. D., M. A. Roy, J. J. O'Neill, and T. E. Devine. 1988. Fatty acids, antibiotic resistance, and deoxyribonucleic acid homology groups of Bradyrhizobium japonicum. Int. J. Syst. Bacteriol. 38:358-361[Abstract/Free Full Text].
16.	Linos, A., and A. Steinbüchel. 1996. Investigations on the microbial breakdown of natural and synthetic rubber, p. 211-219. In Proceedings of the 10th International Biodeterioration and Biodegradation Symposium. VCH-Verlag, Weinheim, Germany.
17.	Maidak, B. L., N. Larsen, M. J. McCoughey, R. Overbeek, G. J. Olsen, K. Folgel, J. Blandy, and C. R. Woese. 1994. The Ribosomal Database Project. Nucleic Acids Res. 22:3485-3487[Abstract/Free Full Text].
18.	McCarthy, A. J., and T. Cross. 1984. A taxonomic study of Thermomonospora and other monosporic actinomycetes. J. Gen. Microbiol. 130:5-25.
19.	McCarthy, A. J. 1987. Lignocelllulose-degrading actinomycetes. FEMS Microbiol. Rev. 46:145-163.
20.	Miller, L. T. 1982. A single derivatization method for routine analysis of bacterial whole-cell fatty acid methyl esters, including hydroxy acids. J. Clin. Microbiol. 16:584-586[Abstract/Free Full Text].
21.	Minnikin, D. E., A. G. O'Donnel, M. Goodfellow, G. Alberton, M. Ethel, A. Scale, and J. H. Parlayed. 1984. An integrated procedure for the extraction of isoprenoid quinones and polar lipids. J. Microbiol. Methods 2:233-241.
22.	Müller, R.-J. 1996. Mechanistic studies on the biodegradation of polyesters, p. 211-219. In Proceedings of the 10th International Biodeterioration and Biodegradation Symposium. VCH-Verlag, Weinheim, Germany.
23.	Nelson, M., S. P. McCarthy, and R. A. Gross. 1992. Isolation of a Pseudomonas paucimobilis capable of using insoluble cellulose acetate as a sole carbon source. Polym. Mater. Sci. Eng. 67:139-140.
24.	Nishida, H., and Y. Tokiwa. 1992. Distribution of poly( $beta$ -hydroxybutyrate) and poly( $varepsilon$ -caprolactone) degrading microorganisms and microbial degradation behaviour on plastic surfaces. Polym. Mater. Sci. Eng. 67:137-138.
25.	Pagga, U. Biodegradability and compostability of polymeric materials in the context of the European packaging regulation. In Proceedings of the International Conference on Advanced Materials, in press.
26.	Pommer, E. H. 1995. Synthetische organische Materialien, p. 111-150. In H. Brill (ed.), Mikrobielle Materialzerstörung und Materialschutz: Schädigungsmechanismen und Schutzmaßnahmen. Gustav Fischer Verlag, Jena, Germany.
27.	Rainey, F. A., M. Dorsch, H. W. Morgan, and E. Stackebrandt. 1992. 16S rDNA analysis of Spirochaeta thermophila: its phylogenetic position and implications for systematics of the order Spirochaetales. Syst. Appl. Microbiol. 15:197-202.
28.	Rainey, F. A., N. Ward-Rainey, R. M. Kroppenstedt, and E. Stackebrandt. 1996. The genus Nocardiopsis represents a phylogenetically coherent taxon and a distinct actinomycete lineage: proposal of Nocardiopsaceae fam. nov. Int. J. Syst. Bacteriol. 46:1088-1092[Abstract/Free Full Text].
29.	Sakai, K., N. Hamada, and Y. Watanabe. 1986. Degradation mechanism of poly(vinyl alcohol) by successive reactions of secondary alcohol oxidase and $beta$ -diketone hydrolase from Pseudomonas sp. Agric. Biol. Chem. 50:989-996.
30.	Sawada, H. ISO standard activities in standardization of biodegradable and/or compostable polymers; development of test methods, definitions. In Proceedings of the International Conference on Advanced Materials, in press.
31.	Staneck, J. L., and G. D. Roberts. 1974. Simplified approach to identification of aerobic actinomycetes by thin-layer chromatography. Appl. Microbiol. 28:226-231[Medline].
32.	Swift, G. 1992. Biodegradable polymers in the environment: are they really biodegradable? Polym. Mater. Sci. Eng. 66:403-404.
33.	Tokiwa, Y., T. Ando, T. Suzuki, and K. Takeda. 1990. Biodegradation of synthetic polymers containing ester bonds. Am. Chem. Soc. Symp. Ser. 433:136-148.
34.	Tsuchii, A., and K. Takeda. 1990. Rubber-degrading enzyme from a bacterial culture. Appl. Environ. Microbiol. 56:1-269[Abstract/Free Full Text].
35.	Witt, U., R.-J. Müller, and W.-D. Deckwer. 1995. New biodegradable polyester-copolymers from commodity chemicals with favourable use properties. J. Environ. Polym. Degrad. 3:215-223.
36.	Witt, U., R.-J. Müller, and W.-D. Deckwer. 1996. Evaluation of the biodegradability of copolyesters containing aromatic compounds by investigations of model oligomers. J. Environ. Polym. Degrad. 4:9-20.
37.	Witt, U., R.-J. Müller, and W.-D. Deckwer. 1996. Studies on sequence distribution of aliphatic/aromatic copolyesters by high-resolution ¹³C nuclear magnetic resonance spectroscopy for evaluation of biodegradability. Makromol. Chem. Phys. 197:1525-1535.
38.	Witt, U., R.-J. Müller, and W.-D. Deckwer. 1997. Biodegradation behaviour and material properties of aliphatic/aromatic polyesters of commercial importance. J. Environ. Polym. Degrad. 5:81-89.