| Literature DB >> 28030589 |
Nural N Cokcetin1, Matthew Pappalardo1,2, Leona T Campbell3, Peter Brooks2, Dee A Carter3, Shona E Blair1, Elizabeth J Harry1.
Abstract
Most commercially available therapeutic honey is derived from flowering Leptospermum scoparium (manuka) plants from New Zealand. Australia has more than 80 Leptospermum species, and limited research to date has found at least some produce honey with high non-peroxide antibacterial activity (NPA) similar to New Zealand manuka, suggesting Australia may have a ready supply of medical-grade honey. The activity of manuka honey is largely due to the presence of methylglyoxal (MGO), which is produced non-enzymatically from dihydroxyacetone (DHA) present in manuka nectar. The aims of the current study were to chemically quantify the compounds contributing to antibacterial activity in a collection of Australian Leptospermum honeys, to assess the relationship between MGO and NPA in these samples, and to determine whether NPA changes during honey storage. Eighty different Leptospermum honey samples were analysed, and therapeutically useful NPA was seen in samples derived from species including L. liversidgei and L. polygalifolium. Exceptionally high levels of up to 1100 mg/kg MGO were present in L. polygalifolium honey samples sourced from the Northern Rivers region in NSW and Byfield, QLD, with considerable diversity among samples. There was a strong positive relationship between NPA and MGO concentration, and DHA was present in all of the active honey samples, indicating a potential for ongoing conversion to MGO. NPA was stable, with most samples showing little change following seven years of storage in the dark at 4°C. This study demonstrates the potential for Australian Leptospermum honey as a wound care product, and argues for an extension of this analysis to other Leptospermum species.Entities:
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Year: 2016 PMID: 28030589 PMCID: PMC5193333 DOI: 10.1371/journal.pone.0167780
Source DB: PubMed Journal: PLoS One ISSN: 1932-6203 Impact factor: 3.240
Methylglyoxal (MGO) and dihydroxyacetone (DHA) levels in Australian Leptospermum honey samples.
| Region | No. of samples tested | MGO | DHA | |||
|---|---|---|---|---|---|---|
| Range | Mean ± SD | Range | Mean ± SD | |||
| Central VIC | 2 | 222–262 | 242 ± 28 | 775–1092 | 934 ± 224 | |
| Central VIC | 1 | NA | 14 ± 0 | NA | 0 ± 0 | |
| Northern Rivers NSW | 1 | NA | 583 ± 9 | NA | 1485 ± 33 | |
| Multifloral | Hunter NSW | 1 | NA | 10 ± 5 | NA | 0 ± 0 |
| Northern Rivers NSW | 1 | NA | 5 ± 1 | NA | 12 ± 17 | |
| Northern Rivers NSW | 5 | 208–704 | 361 ± 205 | 226–882 | 454 ± 282 | |
| Multifloral | Northern Rivers NSW | 13 | 8–362 | 113 ± 127 | 61–818 | 246 ± 231 |
| Byfield QLD | 1 | NA | 1100 ± 57 | NA | 2182 ± 150 | |
| Northern Rivers NSW | 28 | 146–1118 | 628 ± 243 | 157–3425 | 2042 ± 971 | |
| Multifloral | Northern Rivers NSW | 12 | 0–526 | 313 ± 149 | 0–1262 | 689 ± 459 |
| Northern Rivers NSW | 4 | 407–430 | 419 ± 10 | 427–736 | 628 ± 138 | |
| Unspecified | Murraylands SA | 1 | NA | 0 ± 0 | NA | 0 ± 0 |
| Northern Rivers NSW | 6 | 418–836 | 519 ± 158 | 206–1705 | 1205 ± 556 | |
| Stradbroke Island QLD | 1 | NA | 835 ± 36 | NA | 2343 ± 131 | |
| Unknown | 3 | 126–995 | 560 ± 5 | 79–501 | 255 ± 219 | |
aNSW: New South Wales, QLD: Queensland, SA: South Australia, TAS: Tasmania, VIC: Victoria
bMGO: methylglyoxal
cDHA: dihydroxyacetone. NA: not applicable.
Hydroxymethylfurfural (HMF) concentrations in Australian Leptospermum honey collected between 1998 and 2007.
| Year of collection | No. samples tested | HMF | |
|---|---|---|---|
| Mean ± SD | Range | ||
| 1998 | 1 | 143 | NA |
| 2002 | 7 | 49 ± 26 | 4–81 |
| 2003 | 3 | 21 ± 6 | 16–27 |
| 2004 | 5 | 18 ± 7 | 11–29 |
| 2005 | 43 | 14 ± 8 | 0–52 |
| 2006 | 18 | 12 ± 12 | 12–33 |
| 2007 | 2 | 17 ± 2 | 15–18 |
*HMF: hydroxymethylfurfural.
NA: not applicable.
Non-peroxide antibacterial activity of Australian Leptospermum honeys.
| Geographic region | No. of samples | Mean NPA | |
|---|---|---|---|
| Central VIC | 2 | 0 ± 0 | |
| Central VIC | 1 | 0 ± 0 | |
| Northern Rivers NSW | 1 | 18.5 ± 0.2 | |
| Hunter NSW | 1 | 0 ± 0 | |
| Northern Rivers NSW | 1 | 0 ± 0 | |
| Northern Rivers NSW | 5 | 12.2 ± 8 | |
| Northern Rivers NSW | 13 | 2.8 ± 5.4 | |
| Byfield QLD | 1 | 22.9 ± 4.4 | |
| Northern Rivers NSW | 28 | 18.9 ± 5.4 | |
| Northern Rivers NSW | 12 | 11.8 ± 6.2 | |
| Northern Rivers NSW | 4 | 14.8 ± 0.4 | |
| Unspecified | Murraylands SA | 1 | 0 ± 0 |
| Northern Rivers NSW | 6 | 17 ± 3.3 | |
| Stradbroke Island QLD | 1 | 21.9 ± 1.2 | |
| Unknown | 3 | 15.3 ± 13.5 |
aNSW: New South Wales, QLD: Queensland, SA: South Australia, TAS: Tasmania, VIC: Victoria
bNPA: non-peroxide activity.
Fig 1Relationship between methylglyoxal and non-peroxide activity in Australian Leptospermum honeys.
Positive linear correlation between methylglyoxal (MGO) concentration and mean-squared non-peroxide activity (NPA) in Australian Leptospermum honey samples (n = 80) represented by diamond markers; green: MGO >800 mg/kg (NPA >20%), blue: MGO 260–800 mg/kg (NPA 10–20%), red: MGO <260 mg/kg (NPA <10%). Clover honey (purple triangle) served as a negative control with no detectable MGO or NPA, and New Zealand manuka honey (yellow square) and MedihoneyTM (orange circle) both served as the positive controls.
Fig 2Non-peroxide activity (NPA) of Australian Leptospermum honey samples tested seven years apart.
Australian Leptospermum honey samples (n = 61) identified by Irish et al. (2011) as having NPA. Dark grey boxes represent the NPA determined for the honeys at the time of collection (tested 2006–07). Light grey triangles represent NPA tested seven years post-collection in 2014, following storage of the samples in the dark at 4°C.