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	<front>
		<journal-meta>
			<journal-id journal-id-type="publisher-id">pnut</journal-id>
			<journal-id journal-id-type="allenpress-id">pnut</journal-id>
			<journal-title>Peanut Science</journal-title>
			<issn pub-type="ppub">0095-3679</issn>
			<issn pub-type="active">0095-3679</issn>
			<publisher>
				<publisher-name>American Peanut Research and Education Society</publisher-name>
			</publisher>
		</journal-meta>
		<article-meta>
			<article-id pub-id-type="doi">10.3146/i0095-3679-21-2-15</article-id>
			<article-categories>
				<subj-group subj-group-type="heading">
					<subject>Articles</subject>
				</subj-group>
			</article-categories>
			<title-group>
				<article-title><italic>In Vitro</italic> Reproductive Development of a Diploid Wild Species, <italic>Arachis duranensis</italic><xref ref-type="fn" rid="fn1"><sup>1</sup></xref></article-title>
			</title-group>
			<contrib-group>
				<contrib contrib-type="author" xlink:type="simple">
					<name name-style="western">
						<given-names>Q. L.</given-names><x xml:space="preserve"> </x>
						<surname>Feng</surname>
					</name><x xml:space="preserve">, </x>
				</contrib>
				<contrib contrib-type="author" xlink:type="simple">
					<name name-style="western">
						<given-names>H. E.</given-names><x xml:space="preserve"> </x>
						<surname>Pattee</surname>
					</name>
					<xref ref-type="corresp" rid="cor1">&ast;</xref><x xml:space="preserve">, and </x>
				</contrib>
				<contrib contrib-type="author" xlink:type="simple">
					<name name-style="western">
						<given-names>H. T.</given-names><x xml:space="preserve"> </x>
						<surname>Stalker</surname>
					</name>
					<xref ref-type="aff" rid="aff2"><sup>2</sup></xref>
				</contrib>
				
					<aff id="aff2">
					<label><sup>2</sup></label>Grad. Res. Asst., Dept. of Crop Science; Res. Chem., USDA-ARS, Dept. of Botany and Prof., Dept. of Crop Science, North Carolina State Univ., Raleigh, NC 27695-7625
				</aff>
			</contrib-group>
			<author-notes>
				<fn fn-type="fn" id="fn1">
					<p><sup>1</sup>This research was partially supported by the North Carolina Agric. Res. Serv., Raleigh, NC 27695-7643 and the Peanut CRSP, USAID grant DAN-4048-G-SS-2065-00. Recommendations neither represent an official position nor policy of the NCARS or USAID.</p>
				</fn>
				<corresp id="cor1">&ast;Corresponding author.</corresp>
			</author-notes>
			<pub-date pub-type="ppub">
				<month>7</month>
				<year>1994</year>
			</pub-date>
			<volume>21</volume>
			<issue>2</issue>
			<fpage>139</fpage>
			<lpage>143</lpage>
			<history>
				<date date-type="accepted">
					<day>3</day>
					<month>11</month>
					<year>1994</year>
				</date>
			</history>
			<permissions>
				<copyright-statement>American Peanut Research and Education Society</copyright-statement>
				<copyright-year>1994</copyright-year>
				<copyright-holder>American Peanut Research and Education Society</copyright-holder>
			</permissions>
			<related-article related-article-type="pdf" xlink:href="i0095-3679-21-2-15.pdf" xlink:type="simple"></related-article>
			<abstract>
				<title>Abstract</title>
				<p>Embryo abortion at an early stage of reproductive development is a major impediment for introgressing germplasm from wild to cultivated species of <italic>Arachis</italic> by interspecific hybridization. Ovule and embryo culture techniques have been used to rescue aborting hybrid embryos, but increased efficiency and recovery of very young tissues are still needed. The objective of this study was to induce growth and differentiation of <italic>A. duranensis</italic> proembryos. Seven-, 10-, and 14-d-old peg tips were cultured on a modified basal medium containing MS and B<sub>5</sub> media combinations with 16 combination treatments using three growth regulators&mdash;1-naphthaleneacetic acid, gibberellic acid, and 6-benzylaminopurine&mdash;each at four levels. The results showed that seeds could be obtained <italic>in vitro</italic> by peg tip culture of four- to 16-celled proembryos. The favorable concentration ranges of growth regulators for pod formation and embryo development were 0.5-2.0 mg/L NAA, 0.05-0.5 mg/L GA<sub>3</sub>, and 0.05-0.2 mg/L 6-BAP. Over all three selected ages of pegs, the three best combinations of growth regulators resulted in 4.8, 4.7, and 3.5% pod formation, respectively.</p>
			</abstract>
			<kwd-group>
				<title>Key Words</title>
				<kwd>Embryo</kwd><x xml:space="preserve">; </x><x xml:space="preserve">, </x>
				<kwd>pod</kwd><x xml:space="preserve">; </x><x xml:space="preserve">, </x>
				<kwd>peg</kwd><x xml:space="preserve">; </x><x xml:space="preserve">, </x>
				<kwd><italic>in vitro</italic> culture</kwd><x xml:space="preserve">; </x><x xml:space="preserve">, </x>
				<kwd>tissue culture</kwd><x xml:space="preserve">; </x><x xml:space="preserve">, </x>
				<kwd>peanut</kwd><x xml:space="preserve">; </x><x xml:space="preserve">, </x>
				<kwd><italic>Arachis</italic></kwd><x xml:space="preserve">; </x><x xml:space="preserve">, </x>
				<kwd><italic>Arachis duranensis</italic></kwd><x xml:space="preserve">; </x><x xml:space="preserve">, </x>
				<kwd>wild species</kwd>
			</kwd-group>
			<counts>
				<page-count count="5"></page-count>
			</counts>
		</article-meta>
	</front>
</article>
