4A) of the galactoarabinoglucuronoxylan were in good agreement with the results of the linkage analysis. Thus, its spectrum is dominated by five signals of the internal (1 → 4)-linked β-d-Xylp units of the
main chain, with resonances at δ 101.9 (C-1), δ 75.8 (C-4), δ 74.1 (C-3), δ 72.8 (C-2), δ 63.3 (C-5). Their coupled Bcl-2 inhibitor hydrogens were seen in the HSQC experiment, at δ 5.12, 4.42, 4.21, 3.93 and δ 4.75/4.03 respectively. The branching of the xylan side-chains at O-2 of the main-chain units is demonstrated by the set of signals for 2-O-substituted β-d-Xylp units at δ 101.3 (C-1), 77.9 (O-substituted C-2), 76.4 (O-substituted C-4) and 62.9 (C-5). The signals at δ 97.8 (C-1), 72.0 (C-2), 72.2 (C-3), 81.8 (C-4), 172.6 (C-6, not shown) and 59.0 (4-O-methyl-) clearly indicate the presence of 4-O-Me-α-d-GlcpA. A weak resonance at low field in δ 108.2 is of an anomeric carbon of α-l-Araf units. The signals of Arap and Galp could not be observed in the spectrum due to their content, which is too low to be identified by 13C NMR spectroscopy. The assignments are in agreement with published literature data ( Odonmazig et al., 1990 and Shatalov et al., 1999). The eluted fraction on 300 kDa membrane selleck chemical (fraction STK-300E) showed a homogeneous elution profile on HPSEC analysis (Fig. 3B) and was composed of rhamnose (2.0%), arabinose (31.5%), xylose (43.5%),
galactose (14.5%), glucose (2.5%) and uronic acid (6.0%). In addition to five resonances of the (1 → 4)-linked β-d-Xylp ring of the main chain of a xylan, the 13C
NMR spectrum of fraction STK-300E ( Fig. 4B) also showed six intense signals at δ 104.3, 77.6, 74.5, 73.4, 71.9 and 60.8, corresponding to carbons 1, 4, 5, 3, 2, 6 of (1 → 4)-linked β-d-Galp units ( Tanaka et al., 2010). This was indicative of a mixture of polysaccharides with different chemical structures, but with the same molar mass. Thereafter, fraction STK-300E was subjected to treatment Idoxuridine with Fehling solution, giving rise to fractions SF (Fehling supernatant) and PF (Fehling precipitate). This strategy was highly efficient in separating the two polymers, as could be seen by their monosaccharide composition. While fraction SF is composed mainly by arabinose (21.6%) and galactose (46%), indicating the presence of an arabinogalactan, fraction PF is composed of arabinose (22.0%), xylose (62.0%), galactose (5.0%) and uronic acid (11.0%), indicating the presence of the galactoarabinoglucuronoxylan. Their elution profiles on HPSEC are demonstrated in Fig. 2B, with molar mass of 22,000 g/mol (dn/dc = 0.193) for PF. Monosaccharide analysis of carboxy-reduced PF revealed that the uronic acid was represented by glucuronic acid (4.4%) and its 4-O-methyl-derivative (6.6%). Methylation analysis ( Table 1) demonstrated that the galactoarabinoglucuronoxylan present in fraction PF is more branched (∼36.5%) than that present in fraction STK-1000R.