Lysozyme as an aid in preventing stuck wine fermentations

Hetz, Uri

22 June 2001

To provide a possible alternative for the antimicrobial action of sulfur dioxide in winemaking, and address the issue of stuck fermentations, I studied the efficacy of chicken lysozyme (EC 3.2.1.17) as an antimicrobial in grape juice. Two different forms of lysozyme were used: native lysozyme (NL), that is known to be an effective inhibitor of lactic acid bacteria in wine, and partially unfolded lysozyme (PUL), that has been reported to have antimicrobial activity against both Gram-positive and Gram-negative bacteria. Lactobacillus kunkeei and Acetobacter pasteurianus, two bacteria associated with the induction of stuck fermentations were used in the experiments. Chardonnay and Pinot Noir juices were inoculated with L. kunkeei and two days later with yeast strain EC1118 and then incubated for 10 days. The addition of 250ppm of either NL or PUL reduced populations of L. kunkeei to less than 10 CFU/mL in 24 hours while in inoculated grape juice that did not contain any lysozyme, the bacteria grew to 10⁹ CFU/mL within two days. Grape juices supporting the growth of L. kunkeei developed up to 14 times more volatile acidity (VA) than the control or either of the lysozyme treatments. No differences were observed in the antimicrobial action of NL and PUL or in their effects on the composition of the wine. / Graduation date: 2002

Lysozyme

Wine and wine making

Fermentation

Efficacy of Lysozyme as an Alternative to Antibiotics for Broiler Chickens

Gong, Ming

21 March 2014

Antibiotics have been included in poultry feeds to improve growth performance. However, it is a concern that pathogens have become increasingly resistant to antibiotics. Lysozyme is a potential replacement for antibiotics. A trial with or without heat stress was conducted to investigate different inclusion levels (0, 50, 100 and 200ppm) of lysozyme on broiler chickens. Another two trials were conducted using clean or used litter to determine the effect of 100 ppm lysozyme on broiler chickens in each period of the growth cycle. Birds fed the 50 ppm treatment had heavier weight than birds fed the 200 ppm treatment on day 35 (P<0.05). When used litter was provided, feeding lysozyme to birds from days 5-14 and throughout the trial reduced the number of E. coli in the ileum compared with feeding antibiotic to birds (P<0.05). Dietary lysozyme positively influences bacterial numbers in the gastrointestinal tract of broiler chickens.

lysozyme

broiler chickens

growth

microbiota

NMR-based structural and dynamical studies on non-native variants of hen egg white lysozyme

Schlörb, Christian.

Unknown Date

Frankfurt (Main), University, Diss., 2007.

Influence of amorphous adjuvants on the enzymatic activity of spray dried catalase and lysozyme /

Bögelein, Jürgen.

January 2008

Zugl.: Erlangen, Nürnberg, University, Diss., 2008.

Creation of a site-directed mutant of hen egg white lysozyme working toward site-specific oxidation as it relates to protein structure /

Mensah, Eric.

January 2009

Thesis (M.S.)--Youngstown State University, 2009. / Includes bibliographical references (leaves 60-63). Also available via the World Wide Web in PDF format.

Conformational dynamics and intermediates in the folding pathway of T4 lysozyme /

Gillespie, D. Blake,

January 1999

Thesis (Ph. D.)--University of Oregon, 1999. / Typescript. Includes vita and abstract. Includes bibliographical references (leaves 101-110). Also available for download via the World Wide Web; free to University of Oregon users. Address: http://wwwlib.umi.com/cr/uoregon/fullcit?p9957566.

Sedimentation equilibria in nonideal solutions a comparison of three approximations for polydisperse solutes and the self-association of muramidase at 25C̊, pH 7.0, and I = 0.20 /

Deonier, Richard C.,

January 1970

Thesis (Ph. D.)--University of Wisconsin--Madison, 1970. / Typescript. Vita. eContent provider-neutral record in process. Description based on print version record. Includes bibliography.

Determination of folding reversibility of lysozyme crystals using microcalorimetry

Elkordy, Amal A., Forbes, Robert T., Barry, Brian W.

January 2013

Yes

Antimicrobial activity of nisin and hen lysozyme

Jaczynski, Jacek

16 November 1998

Varying concentrations of the food preservatives nisin and lysozyme were adsorbed onto glass surfaces chemically modified to exhibit different degrees of hydrophobicity. The antimicrobial activity of the adsorbed preservatives was evaluated by documenting the ability of Listeria monocytogenes to adhere and grow on the glass surfaces. A bioluminescence protocol was developed to effectively enumerate bacterial cells adhered to glass. Lysozyme adsorption onto glass surfaces was monitored by labeling with ¹²⁵I. Results indicated that synergy was present for 0.9/0.1 molecular ratio of nisin/lysozyme. Synergistic effect was increasing gradually with the increase of nisin in the ratios tested. This trend was observed on both surface types. However, the magnitude of synergy was more pronounced on hydrophobic surfaces than on hydrophilic ones. Results from protein radiolabeling showed that lysozyme was adsorbed with higher mass to hydrophilic surfaces than to hydrophobic ones. / Graduation date: 1999

Nisin

Lysozyme

Listeria monocytogenes

Food -- Preservation

Evolutionary Diversification of Protein Functions : From Translation in Prokaryotes to Innate Immunity in Invertebrates / Evolutionäre Diversifikation von Proteinfunktionen: Von Translation in Prokaryoten zur Angeborenen Immunität in Invertebraten

Prusko, Carsten Dietmar

January 2006

With the progress in sequencing of the honey bee genome new data become available which allows the search and identification of genes coding for homologous proteins found in other organism. Two genes coding for c-type lysozymes were identified in the genome of A. mellifera through an online-based BLAST search. Expression of both intron-less genes seems not to be under the regulatory control of either of the two pathways involved in humoral insect immunity, i.e. Toll and Imd, since no NF-&#954;B transcription factor binding sites are found upstream of the genes. The encoded Lys-1 and Lys-2 are 157 and 143 amino acid long, respectively, and share a sequence similarity of 90%. Further in silico analysis revealed a signal peptidase cleavage site at the N-terminus of each amino acid sequence, strongly suggesting a secretion of the enzymes into the surrounding environment of the producing cells. Sequence alignments of both amino acid sequences with other c-type lysozymes identified the highly conserved active site glutamic acid (Glu32) as well as eight highly conserved cysteine residues. However, an important aspartic acid (Asp50) in the active site that helps to stabilize a substrate intermediate during catalysis is replaced by a serine residue in the lysozymes of A. mellifera. The replacement of the active site aspartic acid in the honey bee lysozymes suggests a different catalytic mechanism and/or a different substrate-specificity in respect to other c-type lysozymes. Furthermore, 3D-models of Lys-1 and Lys-2 were generated based on the sequence similarity of A. mellifera lysozymes with other c-type lysozymes. The published 3D structure of the lysozyme from the silkmoth Bombyx mori, which shares the highest sequence similarity of all available structures with A. mellifera lysozymes, was used as template for the construction of the 3D-models. The models of Lys-1 and Lys-2 suggest that both enzymes resemble, in large part, the structure of B. mori lysozyme. In order to identify the set of AMPs in the hemolymph of A. mellifera, hemolymph of immunized bees was analyzed. Applying SDS-polyacrylamide gel electrophoresis and mass spectrometry on hemolymph from immunized bees, three out of the four peptides were identified, i.e. abaecin, defensin 1 and hymenoptaecin. Furthermore, Lys-2 was identified in the hemolymph by mass spectrometry, conclusively demonstrating the presence of a lysozyme in the hemolymph of A. mellifera for the first time. However, the protein levels of Lys-2 were not affected by bacterial injection, suggesting that the gene expression of the putative antibacterial protein is not under the regulatory control of the Imd and/or Toll pathway. Besides the abovementioned antimicrobial peptides, the 76 kDa large transferrin was also identified. Transferrin is an iron-binding protein that has been implicated in innate immunity in the honey bee. Furthermore, the effect of pathogenic dose, the timeline of peptide induction and the age-related accumulation of the aforementioned AMPs were studied. The intensity of expression of the antimicrobial peptides, abaecin, defensin 1, and hymenoptaecin as well as transferrin increased proportionally with the amount of bacteria injected into the hemocoel. No such effect was observed for the protein levels of Lys-2. Furthermore, up-regulation of the three antibacterial peptides and transferrin was observed within the first 24 h following infection with E. coli (gram-). Infection with the gram+ bacterium Micrococcus flavus resulted in high and moderate protein levels for transferrin and abaecin, respectively, whereas hardly any accumulation of hymenoptaecin was observed, indicating that the gene expression of abaecin and transferrin is somehow positively correlated, and would suggest a shared regulatory pathway that differs from that of hymenoptaecin. Although bacterial infections didn’t seem to stimulate the production of Lys-2, different concentrations in the hemolymph were observed in bees of different ages, suggesting a correlation between the expression of Lys-2 and the age-related division of labor of adult worker honey bees, also known as age polyethism. The results further allow a proposed causal connection between the age-dependent accumulation of Lys-2 and the hemolymph titer of the gonotrophic hormone juvenile hormone, which is the “behavioral pacemaker” in adult honey bees. / Mit der fortschreitenden Sequenzierung des Bienengenoms werden staendig neue Daten zur Verfuegung gestellt, die eine gezielte Suche und Identifizierung von homologen Protein in der Honigbiene ermoeglichen. Mittels einer web-basierenden BLAST-Suche konnten im Genom zwei Gene identifiziert werden, welche fuer Lysozyme des C-typs kodieren. Genauere Untersuchung der Genloci konnten zeigten, dass beide Geneabschnitte keine Bindestellen fuer Transkriptionsfaktoren der NF-&#954;B-Familie aufweisen, und daher davon auszugehen ist, dass die Lysozyme-Gene nicht unter der Kontrolle der beiden regulatroischen Pathways Toll bzw. Imd, von denen man annimmt, dass sie die humorale Immunantwort regulieren, stehen. Die beiden Gene lyz1 und lyz2 kodieren ein 157 bzw. ein 143 Aminosaeure langes Protein, welche zu 90% sequenzielle Aehnlichkeiten aufweisen. Durch weitere in silico Analyse der Protein konnten an den N-termini Erkennungssignale der Signalpeptidase gefunden werden, welche darauf schliessen lassen, dass beide Lysozyme in die Zellumgebung sezerniert werden. Mittels Sequenzvergleiche beider A. mellifera Lysozyme mit anderen C-typ Lysozymen konnte die hochkonservierte und fuer den katalytische Aktivitaet essentielle Aminosaeure Glutamat 32 (Glu32), sowie acht konservierte Cysteine identifiziert werden. Erstaunlicherweise fehlt das fuer den katalytischen Mechanismus essentielle Aspartat 50 (Asp50), welches fuer die Stabilizierung von Intermediaerprodukten wichtig ist. In A. mellifera Lysozymen ist dieses Aspartat durch ein Serin substituiert, was darauf schliessen laesst, dass die beiden Enzyme einen anderen Mechanism und/oder eine andere Substratspezifitaet aufweissen als dies fuer die C-typ Familie der Fall ist. In diesem Zusammenhang wurde ein evolutionaerer Pathway vorgesschlagen, der eine moegliche Transition von Serin zu Aspartat erklaert. Schliesslich konnten aufgrund der Sequenzhomologien zu anderen C-typ Lysozyme und anhand von bestehende Strukturen, 3D-Strukturmodelle der beiden Lysozyme erstellt werde. Die Modelle haben gezeigt, dass die Struktur der beide Enzyme groessenteils den Strukturen andere C-typ Lysozyme gleicht. Zur Identifiezung vom AMPs in A. mellifera, wurde die Hemoplymphe immunisierte Bienen elektrophoretisch und massenspektrometrisch analysisiert. Die drei AMPs Abaecin, Defensin 1 und Hymenoptaecin konnten dabei verifiziert werden. Darueber hinaus wurde zum ersten Mal das Lys-2 in der Hemolymphe nachgewiessen. Anders als bei den drei Oben erwaehnten AMPs, wurde das Lys-2 jedoch nicht durch bakterielle Infektion induziert. Die konstitutive Expression des Lys-2 laesst darauf schliessen, dass es nicht, wie bereits erwaehnt, unter der Kontrolle der beiden immunspezifischen, regulatorischen Pathways Toll und Imd steht. Zusaetlich zu den AMPs wurde das 76 kDa grosse Transferrin, ein Eisen-bindendes Protein, identifiziert, welches eine Rolle in der angeborenen Immunitaet zugesprochen wird. Anhand der genauen Bestimmung der Peptide wurde desweiteren der Effekt der bakteriellen Dosis, der Zeitverlauf der Induktion und die alterabhaengige Induktion naeher untersucht. Die Intensitaet der Expression der AMPs Abaecin, Defensin 1 und Hymenoptaecin sowie Transferrin nahm proportional mit der Menge an injezierten Bakterien zu. Die Akkumulation von Lys-2 wurde dagegen nicht beeinflusst. Desweiteren konnte eine Hochregulierung der Expressionslevel der drei AMPs und Transferrin, nach erfolgter Infektion mit E. coli, innerhalb der ersten 24 Stunden beobachtet werden. Infektion mit dem gram+ Bakterium Micrococcus flavus resultiert dagegen in hoch bzw. moderate Expression von Transferin und Abaecin, jedoch war kaum ein Anstieg der Expression von Hymenoptaecin zu verzeichnen. Dies laesst daraus schliessen, dass die Expression von Abaecin und Transferrin positiv korreliert sind und spricht fuer einen gemeinsamen regulatorischen Pathway, der sich von dem des Hymenoptaecin unterscheidet. Trotz der Beobachtung, dass die Expression von Lys-2 nicht durch bakterielle Infection induziert wird, konnten unterschiedliche Expressionsmuster in Bienen unterschiedlichen Alters beobachtet werden, welche auf eine Korrelation zwischen der Expression des Lys-2 und der altersabhaengigen Arbeitsteilung adulter Honigbienen, dem sogenennten Alterspolythismus, schliessen lassen. Aufgrund dessen, koennte man einen kausalen Zusammenhang zwischen der alterabhaengigen Akkumulation des Lys-2 und dem Hemolymphtiter des gonotrophen Juvenilhormons, welches fuer die Verhaltensaenderung adulter Bienen verantwortlich ist, sehen.

Biene

Lysozyme

Immunreaktion

Molekulargenetik

ddc:570