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  <front>
    <journal-meta>
      <journal-id journal-id-type="publisher-id">JAA</journal-id>
      <journal-title-group>
        <journal-title>Journal of Antioxidant Activity</journal-title>
      </journal-title-group>
      <issn pub-type="epub">2471-2140</issn>
      <publisher>
        <publisher-name>Open Access Pub</publisher-name>
        <publisher-loc>United States</publisher-loc>
      </publisher>
    </journal-meta>
    <article-meta>
      <article-id pub-id-type="publisher-id">JAA-20-3478</article-id>
      <article-id pub-id-type="doi">10.14302/issn.2471-2140.jaa-20-3478</article-id>
      <article-categories>
        <subj-group>
          <subject>research-article</subject>
        </subj-group>
      </article-categories>
      <title-group>
        <article-title>Antioxidant Activity of Surinamese Medicinal Plants with Adaptogenic Properties and Correlation with Total Phenolic Contents</article-title>
        <alt-title alt-title-type="running-head">antioxidant activity and total phenolic contents of adaptogenic plants journal id jaa issn 2471-2140</alt-title>
      </title-group>
      <contrib-group>
        <contrib contrib-type="author">
          <name>
            <surname>Dennis</surname>
            <given-names>R.A. Mans</given-names>
          </name>
          <xref ref-type="aff" rid="idm1849573188">1</xref>
          <xref ref-type="aff" rid="idm1849573476">*</xref>
        </contrib>
        <contrib contrib-type="author">
          <name>
            <surname>Priscilla</surname>
            <given-names>Friperson</given-names>
          </name>
          <xref ref-type="aff" rid="idm1849573188">1</xref>
        </contrib>
        <contrib contrib-type="author">
          <name>
            <surname>Jennifer</surname>
            <given-names>Pawirodihardjo</given-names>
          </name>
          <xref ref-type="aff" rid="idm1849573188">1</xref>
        </contrib>
        <contrib contrib-type="author">
          <name>
            <surname>Meryll</surname>
            <given-names>Djotaroeno</given-names>
          </name>
          <xref ref-type="aff" rid="idm1849573188">1</xref>
        </contrib>
      </contrib-group>
      <aff id="idm1849573188">
        <label>1</label>
        <addr-line>Department of Pharmacology, Faculty of Medical Sciences, Anton de Kom University of Suriname, Paramaribo,                  Suriname</addr-line>
      </aff>
      <aff id="idm1849573476">
        <label>*</label>
        <addr-line>Corresponding author</addr-line>
      </aff>
      <contrib-group>
        <contrib contrib-type="editor">
          <name>
            <surname>Jie</surname>
            <given-names>Yin</given-names>
          </name>
          <xref ref-type="aff" rid="idm1849404004">1</xref>
        </contrib>
      </contrib-group>
      <aff id="idm1849404004">
        <label>1</label>
        <addr-line>Institute of Subtropical Agriculture and University of Chinese Academy of Sciences, china</addr-line>
      </aff>
      <author-notes>
        <corresp>Dennis R.A. Mans, Department of Pharmacology, Faculty of Medical Sciences, Anton de Kom University of Suriname, Kernkampweg 5-7, Paramaribo, Suriname. Tel/Fax: +597 441071. Email: <email>dennismans16@gmail.com</email>.</corresp>
        <fn fn-type="conflict" id="idm1849687412">
          <p>The authors have declared that no competing interests exist.</p>
        </fn>
      </author-notes>
      <pub-date pub-type="epub" iso-8601-date="2020-07-17">
        <day>17</day>
        <month>07</month>
        <year>2020</year>
      </pub-date>
      <volume>2</volume>
      <issue>1</issue>
      <fpage>11</fpage>
      <lpage>28</lpage>
      <history>
        <date date-type="received">
          <day>08</day>
          <month>07</month>
          <year>2020</year>
        </date>
        <date date-type="accepted">
          <day>16</day>
          <month>07</month>
          <year>2020</year>
        </date>
        <date date-type="online">
          <day>17</day>
          <month>07</month>
          <year>2020</year>
        </date>
      </history>
      <permissions>
        <copyright-statement>© </copyright-statement>
        <copyright-year>2020</copyright-year>
        <copyright-holder>Dennis R.A. Mans, et al.</copyright-holder>
        <license xlink:href="http://creativecommons.org/licenses/by/4.0/" xlink:type="simple">
          <license-p>This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.</license-p>
        </license>
      </permissions>
      <self-uri xlink:href="http://openaccesspub.org/jaa/article/1403">This article is available from http://openaccesspub.org/jaa/article/1403</self-uri>
      <abstract>
        <p>Plant-based preparations are commonly used in Suriname (South America) as adaptogens. In this study, fifteen alleged adaptogenic Surinamese plants have been assessed for their antioxidant activity (AA), total phenolic contents (TPC), and total flavonoid contents (TFC). The investigated plants were <italic>Anacardium </italic><italic>occidentale</italic>, <italic>Spondias</italic><italic>dulcis</italic>, <italic>Annona </italic><italic>muricata</italic>, <italic>Euterpe oleracea</italic>, <italic>Oenocarpus</italic><italic> bacaba</italic>, <italic>Luffa </italic><italic>acutangula</italic>, <italic>Punica</italic><italic>granatum</italic>, <italic>Malpighia </italic><italic>emarginata</italic>, <italic>Syzygium</italic><italic>aqueum</italic>, <italic>Syzygium</italic><italic>cumini</italic>, <italic>Averrhoa</italic><italic> carambola</italic>, and <italic>Renealmia</italic><italic>alpinia</italic> (fruit); <italic>Hibiscus sabdariffa</italic> (calyx); as well as <italic>Aloe vera</italic> and <italic>Cestrum </italic><italic>latifolium</italic> (leaf). Aqueous extracts   (1 - 3,000 μg/ mL) were prepared. AA was determined by the FRAP and the DPPH assay. TPC and TFC were determined by the Folin-Ciocalteu’s and an AlCl<sub>3</sub> colorimetric method, respectively, using gallic acid (GA) and rutin (R), respectively, as standards. Data are means ± SDs (n ≥ 3; P &lt; 0.05). FRAP values and                        DPPH-scavenging activities correlated positively with each other and with TPC but not with TFC. The preparations from <italic>M. </italic><italic>emarginata</italic>, <italic>A. carambola</italic>, <italic>A. </italic><italic>occidentale</italic>, <italic>O. bacaba</italic>, <italic>C. </italic><italic>latifolium</italic>, and <italic>H. sabdariffa</italic> displayed the highest FRAP values (54 ± 14 to 412 ± 30 µM Fe<sup>2+</sup>/100 μg), DPPH-scavenging activities (IC<sub>50</sub> values of 33 ± 14 to 250 ± 50 μg/mL), and TPC (51 ± 4 to 280 ± 78 µM GAE/100 µg). TFC of all samples were ≤ 10 ± 3 RE/100 µg. The adaptogenic properties of these plants may (partially) be attributed to their high content of antioxidant phenolic compounds and may make them candidates of novel sources of health-promoting antioxidants.</p>
      </abstract>
      <kwd-group>
        <kwd>Suriname</kwd>
        <kwd>medicinal plants</kwd>
        <kwd>adaptogenic properties</kwd>
        <kwd>antioxidant activity</kwd>
        <kwd>total phenolic content</kwd>
        <kwd>total</kwd>
      </kwd-group>
      <counts>
        <fig-count count="5"/>
        <table-count count="2"/>
        <page-count count="18"/>
      </counts>
    </article-meta>
  </front>
  <body>
    <sec id="idm1849394508" sec-type="intro">
      <title>Introduction</title>
      <p>The dependence of humans on oxygen for their metabolism leads to the continuous formation of reactive oxygen-derived species (ROS) in the body as                        by-products of reactions involving oxygen <xref ref-type="bibr" rid="ridm1843101068">1</xref>. ROS can be generated from either endogenous or exogenous sources. Endogenous sources of ROS are cellular organelles where oxygen consumption is high,                   such as mitochondria, peroxisomes, and endoplasmic                  reticulum <xref ref-type="bibr" rid="ridm1843166940">2</xref>. Exogenous sources of ROS are hazardous environmental chemicals which, as shown for the alkylating antineoplastic agent cyclophosphamide, produce free radicals during their metabolic conversion (see, for instance <xref ref-type="bibr" rid="ridm1843174500">3</xref>). Furthermore, in individuals                  with inherited erythrocyte glucose-6-phosphate dehydrogenase deficiency <xref ref-type="bibr" rid="ridm1842956956">4</xref>, the red blood cells provide insufficient NADPH in response to the rate of ROS formation, resulting in the accumulation of ROS, damage to the red blood cells, and hemolytic anemia (see, for instance, <xref ref-type="bibr" rid="ridm1842952636">5</xref>).</p>
      <p>Examples of ROS are superoxide radical                 anion, hydrogen peroxide, peroxyl radicals, and     hydroxyl <xref ref-type="bibr" rid="ridm1843101068">1</xref>. These species play important roles in key physiological functions such as cell signaling and homeostasis <xref ref-type="bibr" rid="ridm1842940516">6</xref><xref ref-type="bibr" rid="ridm1842944044">7</xref>. However, ROS can also attack cellular macromolecules like the nuclear DNA                       and plasma membrane lipids causing cellular                      injury <xref ref-type="bibr" rid="ridm1842941740">8</xref>. Fortunately, the body has both enzymatic antioxidant systems (for instance, superoxide  dismutase, catalase, and glutathione peroxidase) and non-enzymatic mechanisms (for instance, bilirubin and albumin) to help mitigate this damage <xref ref-type="bibr" rid="ridm1842933828">9</xref>. However, when ROS overwhelm these physiological defenses, oxidative stress occurs <xref ref-type="bibr" rid="ridm1842929868">10</xref>. Oxidative stress can lead to lipid peroxidation, cell and tissues toxicity, and several types of genetic damage that eventually could cause genotoxicity, mutagenicity, secondary cancers, and even cell death (see, for instance <xref ref-type="bibr" rid="ridm1842918300">11</xref>). The resulting homeostatic disruption of multiple metabolic processes may eventually result in the development of neoplastic, cardiovascular, diabetic, neurodegenerative, age-related, and inflammatory ailments <xref ref-type="bibr" rid="ridm1842929868">10</xref><xref ref-type="bibr" rid="ridm1842912684">12</xref>.</p>
      <p>In addition to innate defense systems, exogenous antioxidants provided through the diet and/or nutritional supplements may help protect the body from oxidative stress <xref ref-type="bibr" rid="ridm1842909804">13</xref>. Indeed, several studies have suggested that the consumption of compounds rich in antioxidants decreases the risk of developing the             above-mentioned diseases <xref ref-type="bibr" rid="ridm1842921756">14</xref><xref ref-type="bibr" rid="ridm1842881972">15</xref>. An important class of plant-derived antioxidants is represented by phenolic compounds, secondary plant metabolites made up of one or more aromatic ring(s) coupled to one or more hydroxyl group(s) <xref ref-type="bibr" rid="ridm1842876572">16</xref>. Phenolic compounds also help protect plants from pathogens, animal and insect attack, as well as ultraviolet radiation; provide plants their characteristic colors; and contribute to the organoleptic properties of plants <xref ref-type="bibr" rid="ridm1842872900">17</xref>. There are tens of thousands of plant phenolic compounds including the main dietary constituents flavonoids, phenolic acids, and tannins, in addition to coumarins, naphthoquinones, stilbenes, anthraquinones, and lignans <xref ref-type="bibr" rid="ridm1842909804">13</xref><xref ref-type="bibr" rid="ridm1842876572">16</xref>. Their mitigating effect on oxidative stress has been attributed to their ability to eliminate potentially harmful oxidizing free radical species by acting as reducing agents, hydrogen donors, quenchers of singlet oxygen, or chelators of metal ions that catalyze oxidation reactions <xref ref-type="bibr" rid="ridm1842909804">13</xref><xref ref-type="bibr" rid="ridm1842876572">16</xref>.</p>
      <p>Not surprisingly, the interest in plant-derived phenolic compounds with antioxidant activity is on the rise, and many of these compounds are promoted for preventing and treating illnesses and maintaining general well-being (see, for instance, <xref ref-type="bibr" rid="ridm1842852148">18</xref>). Compounds used for the latter purpose have been called adaptogens, an unofficial term that refers to herbal substances that would help fight stress and fatigue and stimulate well-being by increasing the body’s                        ability to adapt and survive <xref ref-type="bibr" rid="ridm1842848548">19</xref>. When considering                the importance of antioxidants to human                            health <xref ref-type="bibr" rid="ridm1842909804">13</xref><xref ref-type="bibr" rid="ridm1842921756">14</xref><xref ref-type="bibr" rid="ridm1842881972">15</xref> and the capacity of plant phenolic compounds to act as antioxidants <xref ref-type="bibr" rid="ridm1842909804">13</xref><xref ref-type="bibr" rid="ridm1842876572">16</xref>, these phytochemicals may well constitute important ingredients of adaptogens.</p>
      <p>The traditional use of plants and plant-based preparations is deeply rooted in the Republic of Suriname (South America), despite the nationwide availability of affordable and accessible allopathic forms of medicine <xref ref-type="bibr" rid="ridm1842845452">20</xref>. Many traditional preparations are also used for promoting general health, to fight stress, and to obtain extra health benefits <xref ref-type="bibr" rid="ridm1842856972">21</xref><xref ref-type="bibr" rid="ridm1842833620">22</xref><xref ref-type="bibr" rid="ridm1842831388">23</xref><xref ref-type="bibr" rid="ridm1842825988">24</xref><xref ref-type="bibr" rid="ridm1842823252">25</xref><xref ref-type="bibr" rid="ridm1842834844">26</xref><xref ref-type="bibr" rid="ridm1842798932">27</xref><xref ref-type="bibr" rid="ridm1842793460">28</xref><xref ref-type="bibr" rid="ridm1842789428">29</xref><xref ref-type="bibr" rid="ridm1842785252">30</xref>, and can therefore be regarded as adaptogens. Thus, these substances may display unusually high antioxidant activity and contain unusually high amounts of phenolic compounds. So far, studies dealing with these subjects have not been carried out. Therefore, it was decided to assess a number of Surinamese plant preparations that may qualify as adaptogens for their antioxidant activity <italic>in vitro</italic> and their total phenolic content. As flavonoids represent an important class of plant phenolics that are also able to scavenge free radicals and inactivate catalytic metal ions <xref ref-type="bibr" rid="ridm1842780212">31</xref>, the plant samples have also been evaluated for their total flavonoid content. The results obtained may provide scientific substantiation for the adaptogenic properties of the plants and may help identify novel natural sources of antioxidants.</p>
    </sec>
    <sec id="idm1849379940" sec-type="materials">
      <title>Materials and Methods</title>
      <sec id="idm1849379508">
        <title>Plant selection and preparation of Plant Extracts</title>
        <p>The plants evaluated in the current study are mentioned in <xref ref-type="table" rid="idm1841904668">Table 1</xref>. They have been selected on the basis of the number of times they have been dealt with in well-known publications on the use of medicinal plants in Suriname <xref ref-type="bibr" rid="ridm1842856972">21</xref><xref ref-type="bibr" rid="ridm1842833620">22</xref><xref ref-type="bibr" rid="ridm1842831388">23</xref><xref ref-type="bibr" rid="ridm1842825988">24</xref><xref ref-type="bibr" rid="ridm1842823252">25</xref><xref ref-type="bibr" rid="ridm1842834844">26</xref><xref ref-type="bibr" rid="ridm1842798932">27</xref><xref ref-type="bibr" rid="ridm1842793460">28</xref><xref ref-type="bibr" rid="ridm1842789428">29</xref><xref ref-type="bibr" rid="ridm1842785252">30</xref>. The plants have been collected in the period between September and November 2019 in rural areas around Suriname’s capital city Paramaribo that had been free from herbicidal or pesticidal use for at least the preceding six months. The collected plants have been authenticated by staff members from the National Herbarium of Suriname. The plant parts of interest (<xref ref-type="table" rid="idm1841904668">Table 1</xref>) were washed with distilled water, air-dried, washed again, macerated, and extracted with distilled water. This was based on the traditional custom to prepare herbal medicinal teas, infusions, and decoctions by extracting, brewing, or boiling leaves, fruits, stembark, roots, or other plant parts with water <xref ref-type="bibr" rid="ridm1842856972">21</xref><xref ref-type="bibr" rid="ridm1842833620">22</xref><xref ref-type="bibr" rid="ridm1842831388">23</xref><xref ref-type="bibr" rid="ridm1842825988">24</xref><xref ref-type="bibr" rid="ridm1842823252">25</xref><xref ref-type="bibr" rid="ridm1842834844">26</xref><xref ref-type="bibr" rid="ridm1842798932">27</xref><xref ref-type="bibr" rid="ridm1842793460">28</xref><xref ref-type="bibr" rid="ridm1842789428">29</xref><xref ref-type="bibr" rid="ridm1842785252">30</xref>. The extracts were filtered, concentrated by freeze-drying, and the material obtained was divided in aliquots of 0.2 g which were stored at -20 <sup>o</sup>C and tested shortly thereafter.</p>
        <table-wrap id="idm1841904668">
          <label>Table 1.</label>
          <caption>
            <title> Plants investigated in the current study, plant part used and method of processing, as well as the most common traditional medical uses in Suriname</title>
          </caption>
          <table rules="all" frame="box">
            <tbody>
              <tr>
                <td colspan="3">
                  <bold> Plant family </bold>
                </td>
                <td>
                  <bold>Plant part used and method of </bold>
                  <bold>processing</bold>
                </td>
                <td>
                  <bold>Most common </bold>
                  <bold>traditional </bold>
                  <bold>adaptogenic</bold>
                  <bold> uses (references)</bold>
                </td>
              </tr>
              <tr>
                <td> Anacardiaceae</td>
                <td colspan="2"> <italic>Anacardium </italic><italic>occidentale</italic>L. (cashew; kasyu)</td>
                <td> Fruit; squeezed, and juice collected at room temperature, filtered, and freeze-dried</td>
                <td> Throat infections             <xref ref-type="bibr" rid="ridm1842831388">23</xref><xref ref-type="bibr" rid="ridm1842825988">24</xref><xref ref-type="bibr" rid="ridm1842834844">26</xref><xref ref-type="bibr" rid="ridm1842793460">28</xref></td>
              </tr>
              <tr>
                <td>Anacardiaceae </td>
                <td colspan="2"><italic>Spondias</italic><italic>dulcis</italic> L.(ambarella; pommesitère)</td>
                <td>Fruit; squeezed, and juice collected at room temperature, filtered, and freeze-dried</td>
                <td>Fever, cough, wounds, sores, burns <xref ref-type="bibr" rid="ridm1842833620">22</xref><xref ref-type="bibr" rid="ridm1842823252">25</xref></td>
              </tr>
              <tr>
                <td>Annonaceae</td>
                <td colspan="2"><italic>Annona </italic><italic>muricata</italic> L.(soursop; zuurzak)</td>
                <td>Fruit; squeezed, and juice collected at room temperature, filtered, and freeze-dried</td>
                <td>Insomnia, tension, anxiety, exam stress, bedwetting <xref ref-type="bibr" rid="ridm1842825988">24</xref><xref ref-type="bibr" rid="ridm1842834844">26</xref><xref ref-type="bibr" rid="ridm1842793460">28</xref><xref ref-type="bibr" rid="ridm1842789428">29</xref></td>
              </tr>
              <tr>
                <td>Arecaceae</td>
                <td colspan="2"><italic>Euterpe oleracea</italic> Mart.(açai; podosiri)</td>
                <td>Fruit; pulp around seeds removed, macerated, and extracted with             distilled water at room temperature, filtered, and freeze-dried</td>
                <td>Anemia, low blood pressure <xref ref-type="bibr" rid="ridm1842789428">29</xref><xref ref-type="bibr" rid="ridm1842785252">30</xref> </td>
              </tr>
              <tr>
                <td>Arecaceae</td>
                <td colspan="2"><italic>Oenocarpus</italic><italic> bacaba</italic> Mart.(turu palm; kumbu)</td>
                <td>Fruit; pulp around seeds removed, macerated, and extracted with                distilled water at room temperature, filtered, and freeze-dried</td>
                <td>Anemia, low blood pressure <xref ref-type="bibr" rid="ridm1842793460">28</xref><xref ref-type="bibr" rid="ridm1842789428">29</xref> </td>
              </tr>
              <tr>
                <td>Asphodelaceae</td>
                <td colspan="2"><italic>Aloe vera</italic> (L.) Burm.f.(aloe; aloë)</td>
                <td>Inner leaves; squeezed, and gel diluted with distilled water at room temperature, filtered, and                  freeze-dried</td>
                <td>Burns, scars, wound infections, skin rash, scars, hair loss,          dandruff, fever, headache                                   <xref ref-type="bibr" rid="ridm1842825988">24</xref><xref ref-type="bibr" rid="ridm1842834844">26</xref><xref ref-type="bibr" rid="ridm1842793460">28</xref><xref ref-type="bibr" rid="ridm1842789428">29</xref><xref ref-type="bibr" rid="ridm1842785252">30</xref></td>
              </tr>
              <tr>
                <td>Cucurbitaceae </td>
                <td colspan="2"><italic>Luffa </italic><italic>acutangula</italic> (L.) Roxb.(ridged gourd; sukwa)</td>
                <td>Fruit; squeezed, and juice collected at room temperature, filtered, and freeze-dried</td>
                <td>Gall bladder                      functioning <xref ref-type="bibr" rid="ridm1842825988">24</xref> </td>
              </tr>
              <tr>
                <td colspan="2">Lythraceae  </td>
                <td><italic>Punica</italic><italic>granatum</italic> L.(pomegranate; granaatappel) </td>
                <td>Fruit; seed pulps removed, macerated, and extracted with distilled water at room temperature, filtered, and freeze-dried</td>
                <td>General health tonic, bleeding gums, lower respiratory tract complaints, diarrhoea <xref ref-type="bibr" rid="ridm1842856972">21</xref><xref ref-type="bibr" rid="ridm1842825988">24</xref><xref ref-type="bibr" rid="ridm1842793460">28</xref></td>
              </tr>
              <tr>
                <td colspan="2">Malpighiaceae </td>
                <td><italic>Malpighia </italic><italic>emarginata</italic> DC. (1753)(acerola; Westindische kers)</td>
                <td>Fruit; squeezed, and juice collected at room temperature, filtered, and freeze-dried</td>
                <td>Flu, sore throat,                 pimples <xref ref-type="bibr" rid="ridm1842793460">28</xref><xref ref-type="bibr" rid="ridm1842789428">29</xref> </td>
              </tr>
              <tr>
                <td colspan="2">Malvaceae</td>
                <td><italic>Hibiscus sabdariffa</italic> L.(roselle; syuru)</td>
                <td>Calyces; macerated, and infusion prepared, filtered, and freeze-dried</td>
                <td>Coughing, microbial infections, skin and hair care <xref ref-type="bibr" rid="ridm1842785252">30</xref></td>
              </tr>
              <tr>
                <td colspan="2">Myrtaceae</td>
                <td><italic>Syzygium</italic><italic>aqueum</italic> (Burm.f.) Alston(watery rose apple; pommerak)</td>
                <td>Fruit; squeezed, and juice collected at room temperature, filtered, and freeze-dried</td>
                <td>Tonic to improve liver and brain functioning <xref ref-type="bibr" rid="ridm1842833620">22</xref><xref ref-type="bibr" rid="ridm1842823252">25</xref></td>
              </tr>
              <tr>
                <td colspan="2">Myrtaceae </td>
                <td><italic>Syzygium</italic><italic>cumini</italic> (L.) Skeels. (jambolan;            dyamun)</td>
                <td>Fruit; squeezed, and juice collected at room temperature, filtered, and freeze-dried</td>
                <td>Anemia, abdominal pain, diarrhoea, coughing up of blood <xref ref-type="bibr" rid="ridm1842831388">23</xref><xref ref-type="bibr" rid="ridm1842825988">24</xref><xref ref-type="bibr" rid="ridm1842834844">26</xref><xref ref-type="bibr" rid="ridm1842793460">28</xref></td>
              </tr>
              <tr>
                <td colspan="2">Oxalidaceae</td>
                <td><italic>Averrhoa</italic><italic> carambola </italic>L.(star fruit; birambi)</td>
                <td>Fruit; squeezed, and juice collected at room temperature, filtered, and freeze-dried</td>
                <td>Fever, respiratory tract complaints,             fungal skin infections <xref ref-type="bibr" rid="ridm1842793460">28</xref></td>
              </tr>
              <tr>
                <td colspan="2">Solanaceae  </td>
                <td><italic>Cestrum </italic><italic>latifolium</italic> Lam.(bitter greens; bitawiwiri) </td>
                <td>Leaves; macerated and extracted with water for 1 h at 70 <sup>o</sup>C, filtered, and freeze-dried </td>
                <td>Anemia, migraine, stress, flu, eye      inflammation, sore throat, pimples,            itching <xref ref-type="bibr" rid="ridm1842825988">24</xref><xref ref-type="bibr" rid="ridm1842793460">28</xref><xref ref-type="bibr" rid="ridm1842789428">29</xref></td>
              </tr>
              <tr>
                <td colspan="2">Zingiberaceae  </td>
                <td><italic>Renealmia</italic><italic>alpinia</italic> (Rottb.) Maas (ink plant; masusa) </td>
                <td>Fruit; pulp extracted at room temperature, filtered, and freeze-dried </td>
                <td>Genital steam baths <xref ref-type="bibr" rid="ridm1842798932">27</xref>  </td>
              </tr>
            </tbody>
          </table>
        </table-wrap>
      </sec>
      <sec id="idm1849306756">
        <title>Drugs and Chemicals</title>
        <p>Iron(III) chloride hexahydrate (FeCl<sub>3</sub> . 6H<sub>2</sub>O), iron(II) sulfate heptahydrate (FeSO<sub>4</sub> . 7H<sub>2</sub>O), and                       2,4,6-Tris(2-pyridyl)-s-triazine (TPTZ), Folin-Ciocalteu reagent, gallic acid, aluminum chloride hexahydrate (AlCl<sub>3</sub> . 6H<sub>2</sub>O), rutin, and 1,1-diphenyl-2-picrylhydrazyl (DPPH) were from Sigma-Aldrich (St. Louis, MO, USA). Ethanol was from Applichem GmbH (Darmstadt, Germany), sodium carbonate (Na<sub>2</sub>CO<sub>3</sub>) from Merck, (Darmstadt, Germany), and sodium acetate (CH<sub>3</sub>COONa) from BDH Laboratory Supplies (Poole, UK). All other chemicals used were from our laboratory stock and were of the highest grade available.</p>
      </sec>
      <sec id="idm1849304668">
        <title>Determination of Antioxidant Activity of Plant Extracts by the Ferric Reducing/Antioxidant Power Assay</title>
        <p>The antioxidant activity of the plant extracts was determined by a spectrophotometric method based on the ability of an antioxidant to reduce a ferric (Fe<sup>3+</sup>) ion from the Fe<sup>3+</sup>-TPTZ complex to the ferrous (Fe<sup>2+</sup>) ion from a Fe<sup>2+</sup>-tripyridyltriazine complex through the donation of an electron at low pH <xref ref-type="bibr" rid="ridm1842777980">32</xref>. The reactions were spectrophotometrically monitored by measuring the change from the colorless Fe<sup>3+</sup>-TPTZ complex to the intensely blue-colored Fe<sup>2+</sup>-tripyridyltriazine complex at a wavelength at 593 nm. Thus, 3 mL freshly prepared ferric reducing/antioxidant power (FRAP) reagent was mixed with 100 µL of a plant extract and 1 mL distilled water. The FRAP reagent consisted of TPTZ 10 mM in HCl, FeCl<sub>3</sub> . 6H<sub>2</sub>O 20 mM, and acetate buffer 300 mM pH 3.6 in the proportion of 1/1/10 (<italic>v/v/v</italic>). </p>
        <p>After thorough mixing and incubation for 30 min in the dark and at room temperature, the absorbance at 593 nm was recorded against a blank consisting of samples where the plant extract was substituted by distilled water. The change in absorbance was                 directly related to the total reducing power of the electron-donating antioxidants present in the plant extracts. These were estimated from a calibration curve constructed from the absorbance of different concentrations of FeSO<sub>4</sub> at 593 nm and expressed as µm Fe<sup>2+</sup> equivalents reduced per 100 μg lyophilized plant extract.</p>
      </sec>
      <sec id="idm1849300132">
        <title>Determination of Antioxidant Activity of Plant Extracts by the 1,1-diphenyl-2-picrylhydrazyl Assay</title>
        <p>The plant extracts were also assessed for antioxidant activity using a DPPH free radical scavenging assay <xref ref-type="bibr" rid="ridm1842806924">33</xref>. This assay is based on the ability of an antioxidant to inactivate the stable DPPH cation free radical following donation of an electron or hydrogen atom. During his process, the violet colored DPPH molecule becomes colorless to pale yellow, which can spectroscopically be monitored at a wavelength 517 nm. Thus, for each plant extract, seven serial dilutions between 1 and 3,000 μg/mL were prepared, and 0.3 mL of each dilution was mixed with 3 mL absolute ethanol and 0.5 mL DPPH solution of 0.5 mM in ethanol. After 90 min in the dark and at room temperature, the absorbance of the solutions was measured at 517 nm against a mixture of 3.3 mL ethanol and 0.5 mL sample as a blank. The control solution consisted of 3.5 mL ethanol and 0.3 mL DPPH solution.</p>
        <p>The percentage antioxidant activity (AA %) of each dilution of each plant extract was determined using the formula:</p>
        <fig id="idm1841790164">
          <graphic xlink:href="images/image1.png" mime-subtype="png"/>
        </fig>
        <p>where Abs<sub>sample</sub> is the absorbance of the plant extract, Abs<sub>blank</sub> the absorbance of the blank, and Abs<sub>control</sub> the absorbance of the control. For each plant extract, the absorbance values of the dilutions were plotted against the corresponding concentrations. From the resulting dose-response curve, IC<sub>50</sub> values were derived, <italic>i.e.</italic>, the concentrations of the plant extracts (in μg/mL) accomplishing a 50% decrease in absorbance when compared to untreated controls. The lower the IC<sub>50</sub> value, the higher the antioxidant activity.</p>
      </sec>
      <sec id="idm1849298980">
        <title>Determination of Total Phenolic Content of Plant Extracts</title>
        <p>The total phenolic content of the extracts                  was determined using the Folin-Ciocalteu’s             method <xref ref-type="bibr" rid="ridm1842801668">34</xref>. The Folin-Ciocalteu reagent is a mixture of phosphomolybdate and phosphotungstate, and the method is based on the transfer of electrons in alkaline medium from phenolic compounds to the phosphomolybdate/phosphotungstate complex to form a blue chromophore that is spectrophotometrically detectable. Thus, each plant extract was dissolved in distilled water to a concentration of 100 μg/mL. Of each extract, an aliquot of 1.0 mL was added to 0.1 mL             Folin-Ciocalteu reagent 1 N, after which 0.9 mL distilled water was added. The mixture was shaken and allowed to react for 5 min at room temperature. Then, 1.0 mL of Na<sub>2</sub>CO<sub>3</sub> 7% (<italic>w/v</italic>) was added. This solution was adjusted with distilled water to a final volume of 3.4 mL and thoroughly mixed. After incubation for 30 min in the dark, the absorbance was read at 765 nm with respect to a blank containing only Folin-Ciocalteu reagent 1 N and Na<sub>2</sub>CO<sub>3</sub> 7% (<italic>w/v</italic>). The total phenolic content of the plant extracts was calculated from the linear equation of a standard curve prepared with gallic acid (1 to 200 μg/mL) and expressed as µM gallic acid equivalents (GAE) per 100 g lyophilized plant extract.</p>
      </sec>
      <sec id="idm1849296820">
        <title>Determination of Total Flavonoid Content of Plant Extracts</title>
        <p>Total flavonoid content of the plant extracts was determined using a previously described aluminum chloride (AlCl<sub>3</sub>) colorimetric method <xref ref-type="bibr" rid="ridm1842738252">35</xref>. This method is based on the formation of acid-stable complexes between AlCl<sub>3</sub> and the hydroxyl groups of flavones and flavonols. Thus, each plant extract was dissolved in distilled water to give samples of 100 μg/mL. A volume of 0.5 mL AlCl<sub>3</sub> 2% (<italic>w/v</italic>) in absolute ethanol was added to 0.5 mL aliquots of each sample, after which 0.5 mL 1 M potassium acetate and 0.5 mL 1 M HCL were added. The mixture was incubated for 10 min at room temperature and the absorbance was measured at 425 nm against a blank of distilled water. A yellow color indicated the presence of flavonoids. Total flavonoid content of the plant extracts was calculated by intrapolation into a standard curve of rutin prepared from serial dilutions of this compound between 0 and 200 µg/L. Data were expressed as mg rutin equivalents (RE) per 100 g lyophilized plant extract.</p>
      </sec>
      <sec id="idm1849312084">
        <title>Data Processing and Statistics</title>
        <p>All experiments have been carried out at least three times in triplicate. Based on the degree of antioxidant activity found, the samples have been classified into those with high, intermediate, and low antioxidant activity. Data (means ± SDs) have been compared using Student’s t test. The relationship between FRAP values and DPPH free radical-scavenging activities, and between FRAP values or DPPH free   radical-scavenging activities and total phenolic contents or total flavonoid contents, were explored using               two-tailed analysis of bivariate correlation. In all cases, P values &lt; 0.05 were taken to indicate statistically significant differences.</p>
      </sec>
    </sec>
    <sec id="idm1849311796" sec-type="results">
      <title>Results</title>
      <sec id="idm1849311508">
        <title>Relationships Between FRAP Values and DPPH free Radical-scavenging Activities, and Between Antioxidant Activities and Phytochemical Contents of the Plant Samples</title>
        <p>In the current study, fifteen plant extracts that are used in Suriname as adaptogens have been assessed for their antioxidant activity, total phenolic content, and total flavonoid content. Using linear regression analysis, a significant positive correlation (p value &lt; 0.001) was found between FRAP values and DPPH free radical-scavenging activities (a correlation coefficient R<sup>2</sup> of about 0.30; <xref ref-type="fig" rid="idm1841780372">Figure 1</xref>).</p>
        <fig id="idm1841780372">
          <label>Figure 1.</label>
          <caption>
            <title> Relationship between DPPH-scavenging activities and FRAP values in the plant extracts</title>
          </caption>
          <graphic xlink:href="images/image2.jpg" mime-subtype="jpg"/>
        </fig>
        <p>Particularly FRAP values of the preparations correlated well with their total phenolic contents (correlation coefficient R<sup>2</sup> of about 0.91; <xref ref-type="fig" rid="idm1841777996">Figure 2</xref>a), those with higher activity having a relatively high phenolic content and those with low activity a relatively low phenolic content (p value &lt; 0.001). Such a good correlation was not found between DPPH free                radical-scavenging activities and total phenolic contents, but there was still a significant positive relationship (p value &lt; 0.001) between both parameters (a correlation coefficient R<sup>2</sup> of about 0.25; <xref ref-type="fig" rid="idm1841777996">Figure 2</xref>b).</p>
        <fig id="idm1841777996">
          <label>Figure 2a.</label>
          <caption>
            <title> Relationship between total phenolic contents and FRAP values in the plant extracts</title>
          </caption>
          <graphic xlink:href="images/image3.jpg" mime-subtype="jpg"/>
        </fig>
        <fig id="idm1841779076">
          <label>Figure 2b.</label>
          <caption>
            <title> Relationship between total phenolic contents and DPPH-scavenging activities in the plant extracts</title>
          </caption>
          <graphic xlink:href="images/image4.jpg" mime-subtype="jpg"/>
        </fig>
        <p>On the other hand, FRAP values and DPPH free radical-scavenging activities did not correlate well with total flavonoid contents. Correlation coefficients R<sup>2</sup> were 0.0012 and 0.0092, respectively (<xref ref-type="fig" rid="idm1841774972">Figure 3</xref>a and <xref ref-type="fig" rid="idm1841774972">Figure 3</xref>b, respectively), indicating a poor correlation between antioxidant activities and total flavonoid contents (p values of 0.904 and 0.594, respectively).</p>
        <fig id="idm1841774972">
          <label>Figure 3a.</label>
          <caption>
            <title> Relationship between total flavonoid contents and FRAP values in the plant extracts</title>
          </caption>
          <graphic xlink:href="images/image5.jpg" mime-subtype="jpg"/>
        </fig>
        <fig id="idm1841776988">
          <label>Figure 3b.</label>
          <caption>
            <title> Relationship between total flavonoid contents and DPPH-scavenging activities in the plant extracts</title>
          </caption>
          <graphic xlink:href="images/image6.jpg" mime-subtype="jpg"/>
        </fig>
      </sec>
      <sec id="idm1849280700">
        <title>FRAP Values and DPPH Free Radical-scavenging Activities, and Total Phenolic and Flavonoid Contents of the Plant Samples</title>
        <p>Based on the degree of antioxidant activity found, the samples have been classified into those with high, intermediate, and low antioxidant activity                     (<xref ref-type="table" rid="idm1841773532">Table 2</xref>).</p>
        <table-wrap id="idm1841773532">
          <label>Table 2.</label>
          <caption>
            <title> FRAP values, DPPH-scavenging activities, total phenolic contents, and total flavonoid contents of the plant extracts investigated in the current study</title>
          </caption>
          <table rules="all" frame="box">
            <tbody>
              <tr>
                <td> Plant species</td>
                <td> FRAP activity(µm Fe<sup>2+</sup> equivalents         reduced per 100 μg                 lyophilized plant extract)</td>
                <td>DPPH activity(IC<sub>50</sub> in μg/mL)</td>
                <td> Total phenolic              content (µM GAE per 100 µg lyophilized plant extract)</td>
                <td> Total flavonoid content (µM RE per100 µg lyophilized plant extract)</td>
              </tr>
              <tr>
                <td colspan="5"> High antioxidant activity</td>
              </tr>
              <tr>
                <td>
                  <italic>M. </italic>
                  <italic>emarginata</italic>
                </td>
                <td>412 ± 30</td>
                <td>33 ± 14</td>
                <td>280 ± 78</td>
                <td>3 ± 0</td>
              </tr>
              <tr>
                <td colspan="5"> </td>
              </tr>
              <tr>
                <td colspan="5">Intermediate antioxidant activity</td>
              </tr>
              <tr>
                <td>
                  <italic>O. bacaba</italic>
                </td>
                <td>165 ± 29</td>
                <td>78 ± 17</td>
                <td>53 ± 2</td>
                <td>4 ± 2</td>
              </tr>
              <tr>
                <td>
                  <italic>A. carambola</italic>
                </td>
                <td>123 ± 13</td>
                <td>133 ± 14</td>
                <td>89 ± 1</td>
                <td>10 ± 3</td>
              </tr>
              <tr>
                <td>
                  <italic>C. </italic>
                  <italic>latifolium</italic>
                </td>
                <td>87 ± 17</td>
                <td>150 ± 0</td>
                <td>83 ± 10</td>
                <td>3 ± 1</td>
              </tr>
              <tr>
                <td>
                  <italic>H. sabdariffa</italic>
                </td>
                <td>63 ± 9</td>
                <td>183 ± 29</td>
                <td>51 ± 4</td>
                <td>4 ± 2</td>
              </tr>
              <tr>
                <td>
                  <italic>A. </italic>
                  <italic>occidentale</italic>
                </td>
                <td>54 ± 14</td>
                <td>250 ± 50</td>
                <td>61 ± 4</td>
                <td>10± 4</td>
              </tr>
              <tr>
                <td colspan="5"> </td>
              </tr>
              <tr>
                <td colspan="5">Low antioxidant activity</td>
              </tr>
              <tr>
                <td>
                  <italic>E. oleracea</italic>
                </td>
                <td>59 ± 12</td>
                <td>617 ± 29</td>
                <td>25 ± 2</td>
                <td>3 ± 0</td>
              </tr>
              <tr>
                <td>
                  <italic>P. </italic>
                  <italic>granatum</italic>
                </td>
                <td>53 ± 4</td>
                <td>400 ± 0</td>
                <td>22 ± 2</td>
                <td>3 ± 0</td>
              </tr>
              <tr>
                <td>
                  <italic>S. </italic>
                  <italic>aqueum</italic>
                </td>
                <td>36 ± 8</td>
                <td>2,533 ± 351</td>
                <td>13 ± 2</td>
                <td>6 ± 2</td>
              </tr>
              <tr>
                <td>
                  <italic>R. </italic>
                  <italic>alpinia</italic>
                </td>
                <td>25 ± 5</td>
                <td>&gt; 3,000</td>
                <td>23 ± 4</td>
                <td>4 ± 1</td>
              </tr>
              <tr>
                <td>
                  <italic>S. </italic>
                  <italic>dulcis</italic>
                </td>
                <td>10 ± 3</td>
                <td>&gt; 3,000</td>
                <td>12 ± 2</td>
                <td>5 ± 1</td>
              </tr>
              <tr>
                <td>
                  <italic>S. </italic>
                  <italic>cumini</italic>
                </td>
                <td>0</td>
                <td>308 ± 8</td>
                <td>25 ± 4</td>
                <td>3 ± 0</td>
              </tr>
              <tr>
                <td>
                  <italic>A. vera</italic>
                </td>
                <td>0</td>
                <td>1,850 ± 650</td>
                <td>22 ± 10</td>
                <td>3 ± 0</td>
              </tr>
              <tr>
                <td>
                  <italic>L. </italic>
                  <italic>acutangula</italic>
                </td>
                <td>0</td>
                <td>&gt; 3,000</td>
                <td>9 ± 3</td>
                <td>4 ± 1</td>
              </tr>
              <tr>
                <td>
                  <italic>A. </italic>
                  <italic>muricata</italic>
                </td>
                <td>0</td>
                <td>&gt; 3,000 </td>
                <td>13 ± 5 </td>
                <td>4 ± 1 </td>
              </tr>
            </tbody>
          </table>
        </table-wrap>
      </sec>
      <sec id="idm1849215220">
        <title>Plant Extracts with high Antioxidant Activity</title>
        <p>The <italic>Malpighia </italic><italic>emarginata</italic> DC fruit extract exhibited the highest antioxidant activity of the 15 plant samples evaluated, <italic>i.e.</italic>, a FRAP value of µM Fe<sup>2+</sup> equivalents reduced per 100 μg lyophilized material and a DPPH free radical-scavenging activity at an IC<sub>50</sub> value of 33 ± 14 μg/mL (<xref ref-type="table" rid="idm1841773532">Table 2</xref>). This preparation also had the highest total phenol content, namely 280 ± 78 µM GAE per 100 µg lyophilized plant material (<xref ref-type="table" rid="idm1841773532">Table 2</xref>). However, its total flavonoid content was relatively low (3 ± 0 RE per 100 µg lyophilized material; <xref ref-type="table" rid="idm1841773532">Table 2</xref>). Thus, the relatively high antioxidant activity of the <italic>M. </italic><italic>emarginata</italic> preparation correlated well with its relatively high total phenolic content but not with its relatively low total flavonoid content.</p>
      </sec>
      <sec id="idm1849212412">
        <title>Plant Extracts with an Intermediate Antioxidant Activity</title>
        <p>The extracts from <italic>Averrhoa</italic><italic> carambola</italic> L., <italic>Anacardium </italic><italic>occidentale</italic> L., and <italic>Oenocarpus</italic><italic> bacaba</italic> Mart. fruit as well as those from <italic>Hibiscus sabdariffa</italic> L calyx and <italic>Cestrum </italic><italic>latifolium</italic> Lam. leaf had intermediate to high FRAP values (54 ± 14 to 165 ± 29 µM Fe<sup>2+</sup> equivalent reduced per 100 μg lyophilized material, respectively; <xref ref-type="table" rid="idm1841773532">Table 2</xref>), and relatively high DPPH free radical-scavenging activities (IC<sub>50</sub> values of 78 ± 17 to 250 ± 50 μg/mL; <xref ref-type="table" rid="idm1841773532">Table 2</xref>). When compared to the <italic>M. </italic><italic>emarginata</italic> sample, these preparations had the second highest total phenolic content, namely 51 ± 4 to 83 ± 10 µM GAE per 100 µg lyophilized plant material (<xref ref-type="table" rid="idm1841773532">Table 2</xref>). Their total flavonoid contents ranged from were 3 ± 1 to 10 ± 3 µM RE per 100 µg lyophilized plant material (<xref ref-type="table" rid="idm1841773532">Table 2</xref>). Thus, the fairly high antioxidant activity of these preparations correlated reasonably well with their intermediate to high total phenolic content but not with their total flavonoid content.</p>
      </sec>
      <sec id="idm1849205428">
        <title>Plant Extracts with a Low Antioxidant Activity</title>
        <p>The extracts from <italic>Euterpe oleracea</italic> Mart., <italic>Aloe vera</italic> (L.) Burm.f., <italic>Punica</italic><italic>granatum</italic> L., <italic>Syzygium</italic><italic>cumini</italic> L., <italic>Renealmia</italic><italic>alpinia</italic> (Rottb.), <italic>Spondias</italic><italic>dulcis</italic> L., <italic>Annona </italic><italic>muricata</italic> L., <italic>Luffa </italic><italic>acutangula</italic> (L.) Roxb, and <italic>Syzygium</italic><italic>aqueum</italic> (Burm.f.) exhibited very low to intermediate FRAP values (0 to 59 ± 12 µM Fe<sup>2+</sup> equivalents reduced per 100 μg lyophilized material; <xref ref-type="table" rid="idm1841773532">Table 2</xref>) and very low to high DPPH free                        radical-scavenging activities (IC<sub>50</sub> values of &gt; 3000 to 308 ± 8 μg/mL; <xref ref-type="table" rid="idm1841773532">Table 2</xref>). Their total phenolic content was on the lower side (9 ± 3 to 25 ± 4 GAE per 100 µg lyophilized plant material; <xref ref-type="table" rid="idm1841773532">Table 2</xref>). Their total flavonoid content ranged from 3 ± 0 to 6 ± 2 µM RE per 100 µg lyophilized material; <xref ref-type="table" rid="idm1841773532">Table 2</xref>). Apparently, the antioxidant activity of these samples partially correlated with their total phenolic content but not very well with their total flavonoid content.</p>
      </sec>
    </sec>
    <sec id="idm1849200244" sec-type="discussion">
      <title>Discussion</title>
      <p>Preparations from <italic>A. </italic><italic>occidentale</italic>, <italic>S. </italic><italic>dulcis</italic>, <italic>A. </italic><italic>muricata</italic>, <italic>E. oleracea</italic>, <italic>O. bacaba</italic>, <italic>L. </italic><italic>acutangula</italic>, <italic>P. </italic><italic>granatum</italic>, <italic>M. </italic><italic>emarginat</italic>a, <italic>S. </italic><italic>aqueum</italic>, <italic>S. </italic><italic>cumini</italic>, <italic>A. carambola</italic>, and <italic>R. </italic><italic>alpinia</italic> fruit; <italic>H. sabdariffa</italic> calyx; as well as <italic>A. vera</italic> and <italic>C. </italic><italic>latifolium</italic> leaf are extensively used in Suriname for their presumed adaptogenic          properties <xref ref-type="bibr" rid="ridm1842856972">21</xref><xref ref-type="bibr" rid="ridm1842833620">22</xref><xref ref-type="bibr" rid="ridm1842831388">23</xref><xref ref-type="bibr" rid="ridm1842825988">24</xref><xref ref-type="bibr" rid="ridm1842823252">25</xref><xref ref-type="bibr" rid="ridm1842834844">26</xref><xref ref-type="bibr" rid="ridm1842798932">27</xref><xref ref-type="bibr" rid="ridm1842793460">28</xref><xref ref-type="bibr" rid="ridm1842789428">29</xref><xref ref-type="bibr" rid="ridm1842785252">30</xref>. In this study, the possibility that a relatively high antioxidant activity and phenolic content are involved in the alleged health-promoting properties of the plants has been investigated using FRAP and DPPH assays as well as Folin-Ciocalteu’s and AlCl<sub>3</sub> colorimetric methods. The results obtained showed a good correlation between FRAP values and DPPH free radical-scavenging activities of the samples, as well as linear relationships between antioxidant activities and total phenolic content. Such a relationship was not found with flavonoid content. Furthermore, the samples from <italic>M. </italic><italic>emarginata</italic>, <italic>A. carambola</italic>, <italic>A. </italic><italic>occidentale</italic>, and <italic>O. bacaba</italic> fruit as well as <italic>C. </italic><italic>latifolium</italic> leaf and <italic>H. sabdariffa</italic> calyx displayed both intermediate to high antioxidant activities and intermediate to high phenolic contents. These findings may account, at least partially, for the presumed adaptogenic properties of these plants. This did not seem to hold true for the samples of <italic>S. </italic><italic>dulcis</italic>, <italic>A. </italic><italic>muricata</italic>, <italic>E. oleracea</italic>, <italic>L. </italic><italic>acutangula</italic>, <italic>P. </italic><italic>granatum</italic>, <italic>S. </italic><italic>aqueum</italic>, <italic>S. </italic><italic>cumini</italic>, and <italic>R. </italic><italic>alpinia</italic> fruit as well as that from <italic>A. vera</italic> leaf. Thus, these plants either cannot be considered ‘genuine’ adoptogens, or their adoptogenic qualities may be attributable to properties other than the capacity to eliminate free radicals.</p>
      <p>The reasonable correlation between FRAP values and DPPH free radical-scavenging activity suggested that both activities were to some degree consistent with each other. This is in accordance with the comparable principles of these assays: the FRAP assay is based on the ability of an antioxidant to reduce Fe<sup>3+</sup> ions to Fe<sup>2+</sup> ions by donating a hydrogen atom <xref ref-type="bibr" rid="ridm1842777980">32</xref>, the DPPH assay on the capacity of an antioxidant to inactivate the stable DPPH cation radical by donating a hydrogen atom or electron <xref ref-type="bibr" rid="ridm1842806924">33</xref>. Therefore, it can be suggested that the antioxidant ingredients in the different plant samples may have some structural and/or biochemical characteristics in common. Indeed, the possibility of structure-activity-relationships accounting for these observations has been mentioned before (see, for instance <xref ref-type="bibr" rid="ridm1842734148">36</xref>).</p>
      <p>The statistically significant positive relationship of both FRAP values and DPPH free radical-scavenging activities with total phenolic contents suggests that phenolics played an important role in the antioxidant activity of the plant samples. This is in accordance with data from many previous studies (see, for instance, references <xref ref-type="bibr" rid="ridm1842727524">37</xref><xref ref-type="bibr" rid="ridm1842722916">38</xref>) suggesting that the antioxidant activities of plant samples were to a considerable extent determined by their phenolic content. On the other hand, the absence of a significant positive relationship of either FRAP values and DPPH free radical-scavenging activities with total flavonoid contents suggests that these ingredients were not major contributors to the antioxidant activities of the plant extracts. Of note, such a poor correlation between antioxidant activity and total flavonoid content has been reported before <xref ref-type="bibr" rid="ridm1842722196">39</xref><xref ref-type="bibr" rid="ridm1842717084">40</xref>.</p>
      <p>The highest total phenolic content and the highest antioxidant activity among the fifteen plants investigated was found for the <italic>M. </italic><italic>emarginata</italic> fruit extract. This finding is in agreement with previous reports mentioning that an aqueous extract of <italic>M. </italic><italic>emarginata</italic> fruit displayed very potent <italic>in vitro</italic> antioxidant activity <xref ref-type="bibr" rid="ridm1842714492">41</xref><xref ref-type="bibr" rid="ridm1842742860">42</xref> and that its antioxidant activity correlated positively with its total phenolic content <xref ref-type="bibr" rid="ridm1842702708">43</xref><xref ref-type="bibr" rid="ridm1842699324">44</xref>. Furthermore, a methanol extract of <italic>M. </italic><italic>emarginata</italic> fruit had the highest antioxidant activity among ten other underutilized fruits of Andaman Islands (India) <xref ref-type="bibr" rid="ridm1842702708">43</xref> and the highest phenolic content among eleven fruits from Ranong Province and local markets in Bangkok (Thailand) <xref ref-type="bibr" rid="ridm1842699324">44</xref>. The antioxidant activity has been associated with, among others, phenolic compounds such as benzoic acid derivatives, phenylpropanoid derivatives, flavonoids, and anthocyanins, in addition to several carotenoids and an abundant amount of ascorbic acid <xref ref-type="bibr" rid="ridm1842742860">42</xref>.</p>
      <p>The antioxidant activities of the extracts from <italic>A. carambola</italic>, <italic>A. </italic><italic>occidentale</italic>, and <italic>O. bacaba</italic> fruit as well as that of <italic>H. sabdariffa</italic> calyx were in the intermediate to high range and these samples - along with that from <italic>C. </italic><italic>latifolium</italic> leaf - had the second highest total phenolic content when compared to <italic>M. </italic><italic>emarginata</italic> fruit. These observations are in accordance with the strong positive correlation found between total phenolic content and antioxidant activity for <italic>A. carambola</italic> fruit <xref ref-type="bibr" rid="ridm1842694500">45</xref>. The current findings are also in agreement with the high antioxidant activity reported for <italic>A. carambola</italic>, <italic>A. </italic><italic>occidentale</italic>, and <italic>O. bacaba</italic> fruit as well as <italic>H. sabdariffa</italic> calyx <xref ref-type="bibr" rid="ridm1842694500">45</xref><xref ref-type="bibr" rid="ridm1842691836">46</xref><xref ref-type="bibr" rid="ridm1842686652">47</xref><xref ref-type="bibr" rid="ridm1842683844">48</xref>. For the A. carambola sample, this was probably attributable to polyphenolic compounds such as gallic acid, syringic acid, p-coumaric acid, epicatechin, isoquercetin, and procyanidin B2 in addition to ascorbic acid <xref ref-type="bibr" rid="ridm1842680244">49</xref>; for A. occidentale fruit preparations to proanthocyanidins, flavonoids, anthocyanins, tannins as well as ascorbic acid <xref ref-type="bibr" rid="ridm1842676716">50</xref>; for <italic>O. bacaba</italic> fruit to various phenolic compounds including flavonoids and anthocyanins <xref ref-type="bibr" rid="ridm1842645532">51</xref>; and for (methanol extracts of) <italic>H. sabdariffa</italic> calyx mainly to flavonoids, anthocyanins, phenylpropanoids, and carotenoids <xref ref-type="bibr" rid="ridm1842641140">52</xref>. </p>
      <p>As mentioned above, the <italic>C. </italic><italic>latifolium</italic> leaf sample also displayed an intermediate to high antioxidant activity and an intermediate total phenolic content in the current study. Unfortunately, to the best of our knowledge, there are no literature data available for comparison with our findings. However, leaf extracts from other <italic>Cestrum</italic> species such as the purple cestrum <italic>C. elegans</italic>, the red cestrum <italic>C. </italic><italic>fasicilatum</italic>, the green cestrum <italic>C. </italic><italic>parqui</italic>, and the night-blooming cestrum <italic>C. </italic><italic>nocturnum</italic> elicited, comparably to that of <italic>C. </italic><italic>latifolium</italic> in the current study, notable antioxidant activity <xref ref-type="bibr" rid="ridm1842639268">53</xref><xref ref-type="bibr" rid="ridm1842634804">54</xref>. Phytochemical analyses revealed that <italic>C. elegans</italic>, <italic>C. </italic><italic>fasicilatum</italic>, and <italic>C. </italic><italic>parqui</italic> leaves were negative for phenolic compounds but positive for relatively high amounts of flavonoids <xref ref-type="bibr" rid="ridm1842634804">54</xref>, whereas methanol extracts of various parts of <italic>C. </italic><italic>nocturnum</italic> contained substantial amounts of both flavonoids and phenols and exhibited notable free radical-scavenging properties <xref ref-type="bibr" rid="ridm1842639268">53</xref>. Thus, the precise involvement of phenolics and flavonoids in the antioxidant activity of the <italic>C. </italic><italic>latifolium</italic> leaf sample remains to be determined.</p>
      <p>The extracts from <italic>E. oleracea</italic>, <italic>P. </italic><italic>granatum</italic>, and <italic>S. </italic><italic>cumini</italic> fruit displayed an intermediate to high antioxidant activity but a low total phenolic content in the current study. These findings are not in accordance with literature data mentioning that these parts of the plants had high antioxidant activity. Indeed, several investigators reported substantial antioxidant activity of, and considerable quantities of phenolics, - particularly anthocyanins - in <italic>E. </italic><italic>olearacea</italic> fruit pulp <xref ref-type="bibr" rid="ridm1842631780">55</xref><xref ref-type="bibr" rid="ridm1842627244">56</xref>; appreciable antioxidant activity and a relatively high phenolic content of <italic>P. </italic><italic>granatum</italic> juice that included, among others, gallic acid, chlorogenic acid, caffeic acid, ellagic acid, catechin, epicatechin,  quercetin and                 rutin <xref ref-type="bibr" rid="ridm1842624364">57</xref><xref ref-type="bibr" rid="ridm1842621844">58</xref>; and meaningful antioxidant activity and significant amounts of phenolics, - particularly anthocyanins and tannins - as well as carotenoids and antioxidant vitamins in the fruit of <italic>S. </italic><italic>cumini</italic><xref ref-type="bibr" rid="ridm1842615076">59</xref><xref ref-type="bibr" rid="ridm1842598692">60</xref>.</p>
      <p>The discrepancy between the relatively low total phenolic contents found for the <italic>E. oleracea</italic>, <italic>P. </italic><italic>granatum</italic>, and <italic>S. </italic><italic>cumini</italic> samples in the current study, and values reported in the literature, could possibly be ascribed, at least in part, to differences in the extraction methods applied. For instance, samples of <italic>P. </italic><italic>granatum</italic> peel, seed, and seed coat displayed much higher antioxidant activities and phenolic contents upon extraction with 0.1 M HCl: ethanol when compared to those extracted with distilled water <xref ref-type="bibr" rid="ridm1842595308">61</xref>. The inconsistency between the intermediate to high antioxidant activity of the samples and their relatively low total phenolic contents suggests that phenolics were not the only or the major contributors to their antioxidant activity, and that other secondary metabolites might be involved in this activity. Markedly, for <italic>E. oleracea</italic> fruit pulp, the two major anthocyanins (cyanidin-3-glucoside and cyanidin-3-rutinoside) reportedly contributed for about 10% to its overall antioxidant activity, signifying that unidentified substances were responsible for the largest part of activity <xref ref-type="bibr" rid="ridm1842589836">62</xref>. Of note, non-phenolic antioxidant secondary metabolites such as volatile oils, carotenoids, polyunsaturated fatty acids, polysaccharides, and vitamins have also been found to be mainly responsible for the antioxidant activities of certain algae <xref ref-type="bibr" rid="ridm1842585372">63</xref>.</p>
      <p>The extracts from <italic>R. </italic><italic>alpinia</italic> fruit and <italic>A. vera</italic> leaves displayed (very) low antioxidant activity and total phenolic contents in the current study. These findings are partially in line with the relatively low antioxidant activity reported for <italic>R. </italic><italic>alpinia</italic> fruit pulp <xref ref-type="bibr" rid="ridm1842581700">64</xref> despite the presence of phenolic compounds, flavonoids, carotenoids, anthocyanins, and vitamins in this part of the plant, some of which are responsible for the yellow color of the pulp and the red-purple color of its peel <xref ref-type="bibr" rid="ridm1842581700">64</xref>. It is possible that these compounds, similarly to those addressed in the preceding paragraph <xref ref-type="bibr" rid="ridm1842595308">61</xref><xref ref-type="bibr" rid="ridm1842589836">62</xref><xref ref-type="bibr" rid="ridm1842585372">63</xref>, did not possess major antioxidant activity, but this supposition must be verified in future studies.</p>
      <p>The very low antioxidant activity of the <italic>A. vera</italic> leaf preparation seen in the current study is at variance with studies reporting high antioxidant activity of a leaf extract of the plant <xref ref-type="bibr" rid="ridm1842576228">65</xref><xref ref-type="bibr" rid="ridm1842574356">66</xref>. This has been ascribed to, among others, flavonoids, tannins, β-carotene, as well as vitamins C and E <xref ref-type="bibr" rid="ridm1842576228">65</xref><xref ref-type="bibr" rid="ridm1842574356">66</xref>. The dissimilarities between the results from the current study and those mentioned in the literature could be due to the often described variability in biological activity of <italic>A. vera</italic> samples caused by differences in the state of maturity and genotype; conditions of cultivation, harvest time, climatic factors, and the method for harvesting <xref ref-type="bibr" rid="ridm1842699324">44</xref><xref ref-type="bibr" rid="ridm1842569892">67</xref>, and/or the method of extraction and the solvent used for      extraction <xref ref-type="bibr" rid="ridm1842565644">68</xref>.</p>
      <p>The samples from <italic>S. </italic><italic>dulcis</italic>, <italic>A. </italic><italic>muricata</italic>, <italic>L. </italic><italic>acutangula</italic>, and <italic>S. </italic><italic>aqueum</italic> fruit had the lowest antioxidant activity and total phenolic content. For the preparations of <italic>S. </italic><italic>dulcis</italic> and <italic>A. </italic><italic>muricata</italic> fruit, these findings are in line with previous observations indicating that the ethanol extracts of <italic>S. </italic><italic>dulcis</italic> and <italic>S. </italic><italic>cumini</italic> fruit indeed displayed a relatively low DPPH radical scavenging activity and total phenolic content in a study with eleven cheap Bangladeshi fruits <xref ref-type="bibr" rid="ridm1842563052">69</xref>. Furthermore, although <italic>A. </italic><italic>muricata</italic> fruit contains phenolic compounds, flavonoids, ascorbic acid, carotenoids, as well as acetogenins with antioxidant activity <xref ref-type="bibr" rid="ridm1842557796">70</xref>, an ethanolic extract of Sri Lankan <italic>A. </italic><italic>muricata</italic> fruit pulp displayed only a moderate antioxidant activity and total phenolic content when compared to, for instance, the Italian <italic>A. </italic><italic>cherimola</italic> as well as pomegranate and mango                    fruits <xref ref-type="bibr" rid="ridm1842553476">71</xref>.</p>
      <p>The current findings with the <italic>L. </italic><italic>acutangula</italic> and <italic>S. </italic><italic>dulcis</italic> samples could tentatively be explained by the dependence of their antioxidant activity and phenolic content on the polarity of the solvent used, extractions with more polar solvents yielding less activity and phenolics <xref ref-type="bibr" rid="ridm1842551964">72</xref><xref ref-type="bibr" rid="ridm1842545916">73</xref>. In this respect, a methanol extract of <italic>L. </italic><italic>acutangula</italic> fruit and several derived apolar fractions displayed appreciable antioxidant activities (which, however, did not correlate with phenolic and flavonoid contents) while the residual aqueous fraction did                  not <xref ref-type="bibr" rid="ridm1842545916">73</xref>. And <italic>S. </italic><italic>aqueum</italic> fruit reportedly displayed notable antioxidant activity <xref ref-type="bibr" rid="ridm1842702708">43</xref> and represented a rich  source of phenolics and flavonoids <xref ref-type="bibr" rid="ridm1842542028">74</xref> including anthocyanidines <xref ref-type="bibr" rid="ridm1842603300">75</xref> but yielded less antioxidant activity and phenolic compounds when extracted with distilled water instead of methanol <xref ref-type="bibr" rid="ridm1842702708">43</xref>.</p>
    </sec>
    <sec id="idm1849133380" sec-type="conclusions">
      <title>Conclusions</title>
      <p>The results from the current study showed that preparations from <italic>M. </italic><italic>emarginata</italic>, <italic>A. carambola</italic>, <italic>A. </italic><italic>occidentale</italic>, and <italic>O. bacaba</italic> fruit as well as <italic>C. </italic><italic>latifolium</italic> leaf and <italic>H. sabdariffa</italic> calyx displayed relatively high antioxidant activity that correlated well with a high phenolic content. These observations may qualify these plants as ‘genuine’ adaptogens and may help account for some of their claimed medicinal properties <xref ref-type="bibr" rid="ridm1842856972">21</xref><xref ref-type="bibr" rid="ridm1842833620">22</xref><xref ref-type="bibr" rid="ridm1842831388">23</xref><xref ref-type="bibr" rid="ridm1842825988">24</xref><xref ref-type="bibr" rid="ridm1842823252">25</xref><xref ref-type="bibr" rid="ridm1842834844">26</xref><xref ref-type="bibr" rid="ridm1842798932">27</xref><xref ref-type="bibr" rid="ridm1842793460">28</xref><xref ref-type="bibr" rid="ridm1842789428">29</xref><xref ref-type="bibr" rid="ridm1842785252">30</xref>. Importantly, these plants may represent novel natural sources of antioxidants and bioactive health-promoting phytochemicals. The samples from <italic>S. </italic><italic>dulcis</italic>, <italic>A. </italic><italic>muricata</italic>, <italic>E. oleracea</italic>, <italic>L. </italic><italic>acutangula</italic>, <italic>P. </italic><italic>granatum</italic>, <italic>S. </italic><italic>aqueum</italic>, <italic>S. </italic><italic>cumini</italic>, and <italic>R. </italic><italic>alpinia</italic> fruit as well as that from <italic>A. vera</italic> leaf displayed relatively low antioxidant activities and phenolic contents. This suggests that these plants should not be considered ‘genuine’ adoptogens. However, the possibility exists that their adoptogenic qualities are attributable to compounds other than phenolic antioxidants such as carotenoids and/or vitamins C and E. It is also possible that the method of extraction - using distilled water instead of, for instance, methanol - was insufficiently efficient to produce phenolic antioxidants. Studies to assess these possibilities in our laboratories are currently in preparation.</p>
    </sec>
    <sec id="idm1849159588">
      <title>Funding</title>
      <p>This study was partially supported by the Suriname Conservation Foundation (project number SCF. 2012.005).</p>
    </sec>
  </body>
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