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1.
During incubation with physiological buffers at 37°, as well as during in vivo maturation, native collagen fibers display a progressive increase in tensile strength and insolubility. This is paralleled by a progressive loss of reducible, intermolecular crosslinks. The experiments described in this paper indicate that nucleophilic addition of lysine and/or hydroxylysine residues to the electrophilic double bond of the reducible crosslinks transforms them into more stable, non-reducible crosslinks. Indeed, modification of lysine/hydroxylysine residues completely blocks this transformation, while modification of his, arg, glu and asp is without effect. On the basis of these and other experiments, tentative structures are proposed for the stable crosslinks.  相似文献   

2.
Biosynthesis of collagen crosslinks   总被引:3,自引:0,他引:3  
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3.
Stable crosslinks of collagen   总被引:1,自引:0,他引:1  
It has recently been proposed that the syndesine crosslinks of collagen possess their unique stability because they can isomerize to a α-keto-amine. Although this type of isomerization is perfectly feasible for α-hydroxy-aldimines like syndesine, the present studies suggest that the amount of α-keto-amine present in some tissues is far too low to account for the observed stability. However, it is possible that the syndesine crosslinks adopt a cyclic hydrogen-bonded conformation. This could present considerable steric hindrance to hydration of the CN bond, rendering this aldimine crosslink much more stable than those with no α-hydroxy group.  相似文献   

4.
Treatment of calf skin insoluble collagen with NaB3H4 followed by acid hydrolysis and ion-exchange chromatography yields a new compound which is prominent in the chromatograms of several collagens. We now describe this compound as reduced N?-hexosylhydroxylysine. It appears to arise by reduction of the Schiff base between the carbonyl moiety of a hexose and the ?-amino group of hydroxylysine; the postulated structure was derived from both high- and low-resolution mass spectrometry and by comparison with synthetic N?-galactosylhydroxylysine. Conceivably, the unreduced compound may be a crosslink, uniting collagen and glycoproteins or proteoglycans in the connective tissue.  相似文献   

5.
Lung parenchymal collagen is highly insoluble, contributing to the architecture and tensile strength of the lung. Insufficient quantities of collagen are extractable by conventional procedures to permit detailed analyses of collagen types and elucidation of injury to the lung. Sonic bursts at low power release monomer collagen chains from purified tropocollagen fibers. This communication describes sonication procedures at pH 5.2 and 3.0 which release approximately 4 and 15%, respectively, of soluble collagen from lung parenchymal tissue. These quantities are approximately 40 and 140 times greater than are obtained by conventional dilute acid solubilization. The soluble chains are apparently intact and suitable for sensitive determinations which will enable investigators to elucidate the composition of lung collagen fibers.  相似文献   

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The aldehydes present in acid-soluble type I collagen react with pyrenebutyrylhydrazine to form various types of complexes under different reaction conditions. These complexes exhibit one or more of three different pyrene fluorescence bands: monomer, excimer, and aggregate fluorescence. Collagen, whose aldehydes have been reduced with NaBH4, does not react with this fluorescent hydrazine, confirming that the hydrazine reacts specifically with aldehyde groups to form hydrazones. The absence of a reaction with pepsin-treated collagen also shows that the fluorescent labels are primarily in the nonhelical terminal telopeptides. Upon dialysis, the pyrene label bound to a saturated aldehyde in an α-chain is lost; whereas that bound to an unsaturated aldehyde remains on the protein. The pyrene monomer fluorescence in the β-chain of old collagen is stronger than that of young collagen. The formation of the pyrene excimer fluorescence implies the proximity of two pyrene molecules, probably attached to two adjacent aldehydes. Upon changing from acidic to neutral pH, both excimer and aggregate fluorescence bands disappear within a few seconds, revealing a very rapid alteration at the telopeptides.  相似文献   

8.
9.
Intermediate labile intermolecular crosslinks in collagen fibres   总被引:8,自引:0,他引:8  
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10.
Rat lung collagen was labelled in vivo by a single intraperitoneal injection of [3H]lysine at several key timepoints in lung development: days 11 (alveolar proliferation), 26 (start of equilibrated growth), 42 (end of equilibrated growth), and 100 (adult lung structure present). The rates of deposition of labelled hydroxylysine and the difunctional, Schiff base-derived crosslinks hydroxylysinonorleucine (HLNL) and dihydroxylysinonorleucine (DHLNL) were quantified. We also measured total lung content of the trifunctional, mature crosslink hydroxypyridinium (OHP) in these same animals. While the relative rates of accumulation of labelled collagen [3H]hydroxylysine differed by a factor of about 6 at the different times of injection of labelled precursor, quantitative and qualitative patterns of collagen crosslinking were very similar at all of the lung developmental stages studied. Furthermore, there was little or no breakdown of the lung collagen pool as defined by the presence of labelled crosslinks; changes in lung DHLNL content could be completely accounted for by its maturation to OHP, regardless of the age of the rats when injected with the radioactive precursor. We conclude that mature, crosslinked collagen in the lungs of rats, which is obligatorily an extracellular pool, is not being degraded at a measurable rate. Therefore, studies of others that have shown apparent high rates of breakdown of newly synthesized collagen in lungs of whole animals using different methods are probably not reflective of the metabolic fate of total lung collagen, and may indicate that degradation of normal lung collagen occurs predominantly or exclusively intracellularly.  相似文献   

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13.
A rapid and inexpensive method was devised for the determination of lysine-derived aldimine crosslink contents in collagen. The aldimines were converted to their secondary amine derivatives by NaBH4 reduction, and the acid or base collagen hydrolysates analysed directly for these derivatives (HLHNL and HLNL). It was found that in native bone, dentin and cartilage collagen fibres, every two tropocollagen molecules are joined by a minimum of one aldimine crosslink. Negligible amounts of HLNL and HNHNL were found in unreduced collagens, indicating that maturation does not involve a simple in vivo reduction of the aldimine crosslinks.  相似文献   

14.
15.
The stabilization of the intermolecular crosslinks of collagen with ageing   总被引:3,自引:0,他引:3  
A J Bailey 《Gerontologia》1969,15(2):65-76
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16.
17.
The biosynthesis in vivo of the two reducible aldimine crosslinks of immature rabbit articular collagen, hydroxylysinohydroxynorleucine and hydroxylysinonorleucine, is demonstrated. The peak amount of crosslink was detected 1–2 weeks following labeling of the cartilage with [14C]lysine. The subsequent diminution which occurred was due primarily to a decrease in the amount of hydroxylysinohydroxynorleucine. Natural reduction of the aldimine crosslinks in vivo did not occur. Glucosylgalactosyl hydroxylysine and galactosylhydroxylysine, in a 1.451.00 ratio, were synthesized. Seventy-three percent of the hydroxylysine residues were glycosylated. [3H]NaBH4 reduction of non-14C-labeled cartilage showed diminished amounts of reducible crosslink with time and the presence of hexosyl lysines and hexosyl hydroxylysines in mature articular cartilage.  相似文献   

18.
An HPLC method for quantifying the 3-hydroxypyridinium crosslinks of collagen is described. It can be applied to crude hydrolysates of all types of connective tissue. Mineralized tissues can be hydrolyzed directly and analyzed without interference from the mineral ions. The hydroxylysyl (HP) and lysyl (LP) forms of hydroxypyridinium residue were resolved on a reverse-phase C18 column using a gradient of acetonitrile in water and 0.01 M n-heptafluorobutyric acid as an ion-pairing agent. The crosslinking amino acids were accurately quantified down to 2 PM (1 ng) injected, by detecting their natural fluorescence with a spectrofluorometer. Tissues in which hydroxypyridinium crosslinks were plentiful included all forms of cartilage, bone, dentin, ligament, tendon, fascia, intervertebral disc, lung, gut, cervix, aorta, and vitreous humor. Among normal tissues, LP, the minor form of the crosslink, was present in significant amounts relative to HP only in bone and dentin. Both crosslinks were essentially absent from skin, cornea, rat tail tendon, and basement membranes.  相似文献   

19.
Age-related changes in the reducible crosslinks of human tendon collagen   总被引:2,自引:0,他引:2  
K Fujii  M L Tanzer 《FEBS letters》1974,43(3):300-302
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20.
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