Enhancement of microspore embryogenesis induction and plantlet regeneration of sweet pepper (Capsicum annuum L.) using putrescine and ascorbic acid
Production of doubled haploid (DH) plants is an efficient tool in genetic and plant breeding programs; however, sweet pepper ( Capsicum annuum L.) is recalcitrant to microspore embryogenesis and DH production. Trying to break the barrier of DH production, three independent experiments were conducted...
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| Veröffentlicht in: | Protoplasma 2019-01, Vol.256 (1), p.13-24 |
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| creator | Heidari-Zefreh, Ali Akbar Shariatpanahi, Mehran E. Mousavi, Amir Kalatejari, Sepideh |
| description | Production of doubled haploid (DH) plants is an efficient tool in genetic and plant breeding programs; however, sweet pepper (
Capsicum annuum
L.) is recalcitrant to microspore embryogenesis and DH production. Trying to break the barrier of DH production, three independent experiments were conducted on microspore embryogenesis of sweet pepper. In the first experiment, the effect of cold (4 °C) and heat (32 °C) pretreatments were investigated on microspore embryogenesis of three genotypes of sweet pepper including “Inspiration F1,” “Maratus F1,” and “Magno F1” cultivars in a factorial design with three replications. Heat shock (32 °C for 7 days), applied to mannitol-starved anthers of “Inspiration F1,” showed higher multinuclear microspore percent, number of multicellular structures, total embryos, cotyledonary embryos, and regenerants. In the second experiment, the effect of different concentrations of putrescine (0, 0.5, 1, 2, and 5 mg l
−1
) was evaluated on microspore embryogenesis of the three aforementioned cultivars of sweet pepper. The highest mean number of multicellular structures, cotyledonary embryos, and regenerants were achieved by applying 0.5–1 mg l
−1
putrescine during the mannitol starvation and heat shock (32 °C) treatments of isolated microspore culture of “Inspiration F1” cultivar. Significant decrease in microspore embryogenesis efficiency was observed when high levels of putrescine (2 and 5 mg l
−1
) were used. Microspore embryogenesis was prevented completely at 5.0 mg l
−1
putrescine. In the third experiment, the effect of different concentrations of ascorbic acid (0, 20, 50, 100, and 200 mg l
−1
) was investigated and the results showed that the application of ascorbic acid (20 and 50 mg l
−1
) during mannitol starvation and heat shock treatment (32 °C) caused remarkable improvement in the number of produced cotyledonary embryos and their regeneration ability compared to control treatment. However, the application of higher levels of ascorbic acid (100 and 200 mg l
−1
) inhibited microspore cell divisions and embryogenesis. In conclusion, the results indicated that both putrescine and ascorbic acid have significant effect on microspore embryogenesis efficiency of sweet pepper when they are used in appropriate concentrations. |
| doi_str_mv | 10.1007/s00709-018-1268-3 |
| format | Article |
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Capsicum annuum
L.) is recalcitrant to microspore embryogenesis and DH production. Trying to break the barrier of DH production, three independent experiments were conducted on microspore embryogenesis of sweet pepper. In the first experiment, the effect of cold (4 °C) and heat (32 °C) pretreatments were investigated on microspore embryogenesis of three genotypes of sweet pepper including “Inspiration F1,” “Maratus F1,” and “Magno F1” cultivars in a factorial design with three replications. Heat shock (32 °C for 7 days), applied to mannitol-starved anthers of “Inspiration F1,” showed higher multinuclear microspore percent, number of multicellular structures, total embryos, cotyledonary embryos, and regenerants. In the second experiment, the effect of different concentrations of putrescine (0, 0.5, 1, 2, and 5 mg l
−1
) was evaluated on microspore embryogenesis of the three aforementioned cultivars of sweet pepper. The highest mean number of multicellular structures, cotyledonary embryos, and regenerants were achieved by applying 0.5–1 mg l
−1
putrescine during the mannitol starvation and heat shock (32 °C) treatments of isolated microspore culture of “Inspiration F1” cultivar. Significant decrease in microspore embryogenesis efficiency was observed when high levels of putrescine (2 and 5 mg l
−1
) were used. Microspore embryogenesis was prevented completely at 5.0 mg l
−1
putrescine. In the third experiment, the effect of different concentrations of ascorbic acid (0, 20, 50, 100, and 200 mg l
−1
) was investigated and the results showed that the application of ascorbic acid (20 and 50 mg l
−1
) during mannitol starvation and heat shock treatment (32 °C) caused remarkable improvement in the number of produced cotyledonary embryos and their regeneration ability compared to control treatment. However, the application of higher levels of ascorbic acid (100 and 200 mg l
−1
) inhibited microspore cell divisions and embryogenesis. In conclusion, the results indicated that both putrescine and ascorbic acid have significant effect on microspore embryogenesis efficiency of sweet pepper when they are used in appropriate concentrations.</description><identifier>ISSN: 0033-183X</identifier><identifier>EISSN: 1615-6102</identifier><identifier>DOI: 10.1007/s00709-018-1268-3</identifier><identifier>PMID: 29922944</identifier><language>eng</language><publisher>Vienna: Springer Vienna</publisher><subject>Acid production ; Anthers ; Ascorbic acid ; Ascorbic Acid - metabolism ; Biomedical and Life Sciences ; Capsicum - genetics ; Capsicum annuum ; Cell Biology ; Cell culture ; Embryogenesis ; Embryonic Development - genetics ; Experiments ; Genotypes ; Heat shock ; Life Sciences ; Mannitol ; Original Article ; Plant breeding ; Plant Sciences ; Putrescine ; Putrescine - metabolism ; Vitamin C ; Zoology</subject><ispartof>Protoplasma, 2019-01, Vol.256 (1), p.13-24</ispartof><rights>Springer-Verlag GmbH Austria, part of Springer Nature 2018</rights><rights>Protoplasma is a copyright of Springer, (2018). All Rights Reserved.</rights><lds50>peer_reviewed</lds50><woscitedreferencessubscribed>false</woscitedreferencessubscribed><citedby>FETCH-LOGICAL-c372t-b5fc8cf357e242b80655805c353e4e658d1a17aa495a592f63c8217d2b5e652a3</citedby><cites>FETCH-LOGICAL-c372t-b5fc8cf357e242b80655805c353e4e658d1a17aa495a592f63c8217d2b5e652a3</cites></display><links><openurl>$$Topenurl_article</openurl><openurlfulltext>$$Topenurlfull_article</openurlfulltext><thumbnail>$$Tsyndetics_thumb_exl</thumbnail><linktopdf>$$Uhttps://link.springer.com/content/pdf/10.1007/s00709-018-1268-3$$EPDF$$P50$$Gspringer$$H</linktopdf><linktohtml>$$Uhttps://link.springer.com/10.1007/s00709-018-1268-3$$EHTML$$P50$$Gspringer$$H</linktohtml><link.rule.ids>314,780,784,27923,27924,41487,42556,51318</link.rule.ids><backlink>$$Uhttps://www.ncbi.nlm.nih.gov/pubmed/29922944$$D View this record in MEDLINE/PubMed$$Hfree_for_read</backlink></links><search><creatorcontrib>Heidari-Zefreh, Ali Akbar</creatorcontrib><creatorcontrib>Shariatpanahi, Mehran E.</creatorcontrib><creatorcontrib>Mousavi, Amir</creatorcontrib><creatorcontrib>Kalatejari, Sepideh</creatorcontrib><title>Enhancement of microspore embryogenesis induction and plantlet regeneration of sweet pepper (Capsicum annuum L.) using putrescine and ascorbic acid</title><title>Protoplasma</title><addtitle>Protoplasma</addtitle><addtitle>Protoplasma</addtitle><description>Production of doubled haploid (DH) plants is an efficient tool in genetic and plant breeding programs; however, sweet pepper (
Capsicum annuum
L.) is recalcitrant to microspore embryogenesis and DH production. Trying to break the barrier of DH production, three independent experiments were conducted on microspore embryogenesis of sweet pepper. In the first experiment, the effect of cold (4 °C) and heat (32 °C) pretreatments were investigated on microspore embryogenesis of three genotypes of sweet pepper including “Inspiration F1,” “Maratus F1,” and “Magno F1” cultivars in a factorial design with three replications. Heat shock (32 °C for 7 days), applied to mannitol-starved anthers of “Inspiration F1,” showed higher multinuclear microspore percent, number of multicellular structures, total embryos, cotyledonary embryos, and regenerants. In the second experiment, the effect of different concentrations of putrescine (0, 0.5, 1, 2, and 5 mg l
−1
) was evaluated on microspore embryogenesis of the three aforementioned cultivars of sweet pepper. The highest mean number of multicellular structures, cotyledonary embryos, and regenerants were achieved by applying 0.5–1 mg l
−1
putrescine during the mannitol starvation and heat shock (32 °C) treatments of isolated microspore culture of “Inspiration F1” cultivar. Significant decrease in microspore embryogenesis efficiency was observed when high levels of putrescine (2 and 5 mg l
−1
) were used. Microspore embryogenesis was prevented completely at 5.0 mg l
−1
putrescine. In the third experiment, the effect of different concentrations of ascorbic acid (0, 20, 50, 100, and 200 mg l
−1
) was investigated and the results showed that the application of ascorbic acid (20 and 50 mg l
−1
) during mannitol starvation and heat shock treatment (32 °C) caused remarkable improvement in the number of produced cotyledonary embryos and their regeneration ability compared to control treatment. However, the application of higher levels of ascorbic acid (100 and 200 mg l
−1
) inhibited microspore cell divisions and embryogenesis. In conclusion, the results indicated that both putrescine and ascorbic acid have significant effect on microspore embryogenesis efficiency of sweet pepper when they are used in appropriate concentrations.</description><subject>Acid production</subject><subject>Anthers</subject><subject>Ascorbic acid</subject><subject>Ascorbic Acid - metabolism</subject><subject>Biomedical and Life Sciences</subject><subject>Capsicum - genetics</subject><subject>Capsicum annuum</subject><subject>Cell Biology</subject><subject>Cell culture</subject><subject>Embryogenesis</subject><subject>Embryonic Development - genetics</subject><subject>Experiments</subject><subject>Genotypes</subject><subject>Heat shock</subject><subject>Life Sciences</subject><subject>Mannitol</subject><subject>Original Article</subject><subject>Plant breeding</subject><subject>Plant Sciences</subject><subject>Putrescine</subject><subject>Putrescine - metabolism</subject><subject>Vitamin C</subject><subject>Zoology</subject><issn>0033-183X</issn><issn>1615-6102</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2019</creationdate><recordtype>article</recordtype><sourceid>EIF</sourceid><sourceid>ABUWG</sourceid><sourceid>AFKRA</sourceid><sourceid>AZQEC</sourceid><sourceid>BENPR</sourceid><sourceid>CCPQU</sourceid><sourceid>DWQXO</sourceid><sourceid>GNUQQ</sourceid><recordid>eNp1kc1q3DAUhUVJaKbTPkA3RZBNunCqH8uWl2VIf2AgmxS6E7J8PVEYS6pkEeY58sKRM2kKhWzuBd3vHEn3IPSRkktKSPsllUK6ilBZUdbIir9BK9pQUTWUsBO0IoTzikr--wy9S-mOECIYEW_RGes6xrq6XqGHK3ernYEJ3Iz9iCdrok_BR8Aw9fHgd-Ag2YStG7KZrXdYuwGHvXbzHmYcYQGifpoUfbqHchogBIj4YqNDsiZPReNyadvLzzgn63Y45DlCMtbBk59OxsfeGqyNHd6j01HvE3x47mv069vVzeZHtb3-_nPzdVsZ3rK56sVopBm5aIHVrJekEUISYbjgUEMj5EA1bbWuO6FFx8aGG8loO7BelCnTfI0ujr4h-j8Z0qwmmwzsy9_A56TKrtqaN7KUNTr_D73zObryuoVqOlKzlhaKHqllhynCqEK0k44HRYlaElPHxFRJTC2JKV40n56dcz_B8KL4G1EB2BFIZeR2EP9d_brrI40Qopo</recordid><startdate>20190101</startdate><enddate>20190101</enddate><creator>Heidari-Zefreh, Ali Akbar</creator><creator>Shariatpanahi, Mehran E.</creator><creator>Mousavi, Amir</creator><creator>Kalatejari, Sepideh</creator><general>Springer Vienna</general><general>Springer Nature B.V</general><scope>CGR</scope><scope>CUY</scope><scope>CVF</scope><scope>ECM</scope><scope>EIF</scope><scope>NPM</scope><scope>AAYXX</scope><scope>CITATION</scope><scope>3V.</scope><scope>7RV</scope><scope>7X7</scope><scope>7XB</scope><scope>88E</scope><scope>88G</scope><scope>8AO</scope><scope>8FE</scope><scope>8FH</scope><scope>8FI</scope><scope>8FJ</scope><scope>8FK</scope><scope>ABUWG</scope><scope>AFKRA</scope><scope>AZQEC</scope><scope>BBNVY</scope><scope>BENPR</scope><scope>BHPHI</scope><scope>CCPQU</scope><scope>DWQXO</scope><scope>FYUFA</scope><scope>GHDGH</scope><scope>GNUQQ</scope><scope>HCIFZ</scope><scope>K9.</scope><scope>KB0</scope><scope>LK8</scope><scope>M0S</scope><scope>M1P</scope><scope>M2M</scope><scope>M7P</scope><scope>NAPCQ</scope><scope>PQEST</scope><scope>PQQKQ</scope><scope>PQUKI</scope><scope>PRINS</scope><scope>PSYQQ</scope><scope>Q9U</scope><scope>7X8</scope></search><sort><creationdate>20190101</creationdate><title>Enhancement of microspore embryogenesis induction and plantlet regeneration of sweet pepper (Capsicum annuum L.) using putrescine and ascorbic acid</title><author>Heidari-Zefreh, Ali Akbar ; Shariatpanahi, Mehran E. ; Mousavi, Amir ; Kalatejari, Sepideh</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-LOGICAL-c372t-b5fc8cf357e242b80655805c353e4e658d1a17aa495a592f63c8217d2b5e652a3</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>2019</creationdate><topic>Acid production</topic><topic>Anthers</topic><topic>Ascorbic acid</topic><topic>Ascorbic Acid - metabolism</topic><topic>Biomedical and Life Sciences</topic><topic>Capsicum - genetics</topic><topic>Capsicum annuum</topic><topic>Cell Biology</topic><topic>Cell culture</topic><topic>Embryogenesis</topic><topic>Embryonic Development - genetics</topic><topic>Experiments</topic><topic>Genotypes</topic><topic>Heat shock</topic><topic>Life Sciences</topic><topic>Mannitol</topic><topic>Original Article</topic><topic>Plant breeding</topic><topic>Plant Sciences</topic><topic>Putrescine</topic><topic>Putrescine - metabolism</topic><topic>Vitamin C</topic><topic>Zoology</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Heidari-Zefreh, Ali Akbar</creatorcontrib><creatorcontrib>Shariatpanahi, Mehran E.</creatorcontrib><creatorcontrib>Mousavi, Amir</creatorcontrib><creatorcontrib>Kalatejari, Sepideh</creatorcontrib><collection>Medline</collection><collection>MEDLINE</collection><collection>MEDLINE (Ovid)</collection><collection>MEDLINE</collection><collection>MEDLINE</collection><collection>PubMed</collection><collection>CrossRef</collection><collection>ProQuest Central (Corporate)</collection><collection>ProQuest Nursing and Allied Health Journals</collection><collection>ProQuest Health & Medical Collection</collection><collection>ProQuest Central (purchase pre-March 2016)</collection><collection>Medical Database (Alumni Edition)</collection><collection>Psychology Database (Alumni)</collection><collection>ProQuest Pharma Collection</collection><collection>ProQuest SciTech Collection</collection><collection>ProQuest Natural Science Collection</collection><collection>Hospital Premium Collection</collection><collection>Hospital Premium Collection (Alumni Edition)</collection><collection>ProQuest Central (Alumni) (purchase pre-March 2016)</collection><collection>ProQuest Central (Alumni)</collection><collection>ProQuest Central</collection><collection>ProQuest Central Essentials</collection><collection>Biological Science Collection</collection><collection>AUTh Library subscriptions: ProQuest Central</collection><collection>ProQuest Natural Science Collection</collection><collection>ProQuest One Community College</collection><collection>ProQuest Central</collection><collection>Health Research Premium Collection</collection><collection>Health Research Premium Collection (Alumni)</collection><collection>ProQuest Central Student</collection><collection>SciTech Premium Collection</collection><collection>ProQuest Health & Medical Complete (Alumni)</collection><collection>Nursing & Allied Health Database (Alumni Edition)</collection><collection>Biological Sciences</collection><collection>Health & Medical Collection (Alumni Edition)</collection><collection>Medical Database</collection><collection>Psychology Database</collection><collection>Biological Science Database</collection><collection>Nursing & Allied Health Premium</collection><collection>ProQuest One Academic Eastern Edition (DO NOT USE)</collection><collection>ProQuest One Academic</collection><collection>ProQuest One Academic UKI Edition</collection><collection>ProQuest Central China</collection><collection>ProQuest One Psychology</collection><collection>ProQuest Central Basic</collection><collection>MEDLINE - Academic</collection><jtitle>Protoplasma</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Heidari-Zefreh, Ali Akbar</au><au>Shariatpanahi, Mehran E.</au><au>Mousavi, Amir</au><au>Kalatejari, Sepideh</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Enhancement of microspore embryogenesis induction and plantlet regeneration of sweet pepper (Capsicum annuum L.) using putrescine and ascorbic acid</atitle><jtitle>Protoplasma</jtitle><stitle>Protoplasma</stitle><addtitle>Protoplasma</addtitle><date>2019-01-01</date><risdate>2019</risdate><volume>256</volume><issue>1</issue><spage>13</spage><epage>24</epage><pages>13-24</pages><issn>0033-183X</issn><eissn>1615-6102</eissn><abstract>Production of doubled haploid (DH) plants is an efficient tool in genetic and plant breeding programs; however, sweet pepper (
Capsicum annuum
L.) is recalcitrant to microspore embryogenesis and DH production. Trying to break the barrier of DH production, three independent experiments were conducted on microspore embryogenesis of sweet pepper. In the first experiment, the effect of cold (4 °C) and heat (32 °C) pretreatments were investigated on microspore embryogenesis of three genotypes of sweet pepper including “Inspiration F1,” “Maratus F1,” and “Magno F1” cultivars in a factorial design with three replications. Heat shock (32 °C for 7 days), applied to mannitol-starved anthers of “Inspiration F1,” showed higher multinuclear microspore percent, number of multicellular structures, total embryos, cotyledonary embryos, and regenerants. In the second experiment, the effect of different concentrations of putrescine (0, 0.5, 1, 2, and 5 mg l
−1
) was evaluated on microspore embryogenesis of the three aforementioned cultivars of sweet pepper. The highest mean number of multicellular structures, cotyledonary embryos, and regenerants were achieved by applying 0.5–1 mg l
−1
putrescine during the mannitol starvation and heat shock (32 °C) treatments of isolated microspore culture of “Inspiration F1” cultivar. Significant decrease in microspore embryogenesis efficiency was observed when high levels of putrescine (2 and 5 mg l
−1
) were used. Microspore embryogenesis was prevented completely at 5.0 mg l
−1
putrescine. In the third experiment, the effect of different concentrations of ascorbic acid (0, 20, 50, 100, and 200 mg l
−1
) was investigated and the results showed that the application of ascorbic acid (20 and 50 mg l
−1
) during mannitol starvation and heat shock treatment (32 °C) caused remarkable improvement in the number of produced cotyledonary embryos and their regeneration ability compared to control treatment. However, the application of higher levels of ascorbic acid (100 and 200 mg l
−1
) inhibited microspore cell divisions and embryogenesis. In conclusion, the results indicated that both putrescine and ascorbic acid have significant effect on microspore embryogenesis efficiency of sweet pepper when they are used in appropriate concentrations.</abstract><cop>Vienna</cop><pub>Springer Vienna</pub><pmid>29922944</pmid><doi>10.1007/s00709-018-1268-3</doi><tpages>12</tpages></addata></record> |
| fulltext | fulltext |
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| ispartof | Protoplasma, 2019-01, Vol.256 (1), p.13-24 |
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| subjects | Acid production Anthers Ascorbic acid Ascorbic Acid - metabolism Biomedical and Life Sciences Capsicum - genetics Capsicum annuum Cell Biology Cell culture Embryogenesis Embryonic Development - genetics Experiments Genotypes Heat shock Life Sciences Mannitol Original Article Plant breeding Plant Sciences Putrescine Putrescine - metabolism Vitamin C Zoology |
| title | Enhancement of microspore embryogenesis induction and plantlet regeneration of sweet pepper (Capsicum annuum L.) using putrescine and ascorbic acid |
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