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1  but not cortisol, corticotropin, or urinary N-telopeptide.
2 's reagent, and immunoassay for cross-linked N-telopeptides.
3  with conventional antibiotics, decreases in N-telopeptides (147.3 +/- 77.5 [mean +/- SEM] versus 95.
4                                        Urine N-telopeptide, a bone resorption marker, levels declined
5                                    Levels of N-telopeptide, a marker of bone resorption, were greater
6                                        Serum N-telopeptide, a marker of osteoclast activity, decrease
7  Measurement of serum levels of cross-linked N-telopeptides, a specific measure of bone resorption ac
8                                 Cross-linked N-telopeptides accounted for two-thirds of the total lys
9 D, parathyroid hormone, osteocalcin, urinary N-telopeptides, albumin, insulin-like growth factor I, a
10             In the upfront group, mean serum N-telopeptide and bone-specific alkaline phosphatase con
11 noline to lysylpyridinoline differed between N-telopeptide and C-telopeptide sites, and between the i
12  0.02, r2 = 0.586, n = 9), and between serum N-telopeptide and total alkaline phosphatase (P < 0.001,
13            Three weeks later, the changes in N-telopeptides and osteocalcin persisted.
14 ne, midtreatment, and posttreatment, urinary N:-telopeptides and serum bone-specific alkaline phospha
15 indirect marker of bone resorption in urine (N:-telopeptide) and 1,25(OH)2D (P < 0.02, r2 = 0.586, n
16                             Urinary calcium, N-telopeptide, and pyridinium cross-links were measured
17           Prior studies showed that a docked N-telopeptide can interact with two adjacent collagen mo
18 serum bone alkaline phosphatase, and urinary N-telopeptide collagen crosslink (NTx) concentrations we
19  of change in the bone turnover marker urine N-telopeptide corrected for urine creatinine (uNTx/Cr) f
20 eocalcin and parathyroid hormone and urinary N-telopeptide, cortisol, and calcium excretion were meas
21 phorous increased at 6 months, whereas urine N-telopeptides decreased.
22 he same sites, but concentrated (85%) at the N-telopeptide end.
23 ium intake was significantly correlated with N-telopeptide in the SED group during bed rest weeks 3 a
24 rence, -30%; 95% CI, -26% to -33%) and urine N-telopeptide levels (mean change, -48% vs 4%; between-g
25 y increased BMD and durably suppressed serum N-telopeptide levels for 12 months.
26                      Urinary measurements of N-telopeptide (Ntx) and serum bone alkaline phosphatase
27 erminal propeptide (P1NP) and urine collagen N-telopeptide (NTx) levels increased with teriparatide t
28 ne formation and resorption, osteocalcin and N-telopeptide (NTX), in patients with AN (n=28) who were
29 hatase and osteocalcin) and bone resorption (N-telopeptide of collagen cross-links); urinalysis; and
30 ly decreased serum levels of osteocalcin and N-telopeptide of collagen cross-links.
31 bone-specific alkaline phosphatase and urine N-telopeptide of collagen.
32                                 Cross-linked N-telopeptide of type 1 collagen (NTx) breakdown, osteoc
33          Urine was analyzed for cross-linked N-telopeptide of type I collagen, a bone resorption mark
34 nal telopeptide of type I collagen and urine N-telopeptide of type I collagen, in all three cell type
35                    Markers of bone turnover, N-telopeptides of type 1 collagen, and bone alkaline pho
36 teocalcin, a marker of bone formation; urine N-telopeptides of type I collagen and free deoxypyridino
37                              Osteocalcin and N-telopeptides of type I collagen were significantly red
38 alcin, and the ratio of urinary cross-linked N:-telopeptides of type 1 collagen to creatinine with al
39 ed osteocalcin (ucOC) and total osteocalcin, N:-telopeptides of type I collagen (NTx), bone-specific
40 escence alone can underestimate the level of N-telopeptide pyridinoline cross-linking.
41                                              N-telopeptide pyridinoline fluorescence was quenched on
42    Residue K(160), located in the nonhelical N-telopeptide region and involved in pyridinoline cross-
43 agen, with the binding region located at the N-telopeptide region of type I collagen.
44 cond year, the bone resorption marker, serum N-telopeptide, rose by 27% in the calcitriol group (P< o
45  pyridinoline cross-linking were identified, N-telopeptide to helix and C-telopeptide to helix.
46  Several peptide combinations arose from the N-telopeptide to helix site, but the main source of pyri
47  bisphosphonate use (yes vs no), and urinary N-telopeptide (uNTx) value (<60 mumol/mol creatinine vs
48             Pyridinolines linking two alpha1(N) telopeptides were a minor component.
49 e than 55%, whereas excretion of crosslinked n-telopeptide, which reflects bone resorption, increased

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