ISOLASI DAN IDENTIFIKASI SENYAWA PENANGKAP RADIKAL 2,2-DIFENIL-1-PIKRILHIDRAZIL DALAM DAUN KELOR (Moringa oleifera, Lamk.)
Free radical is suspected as mediator of various degenerative diseases. Antioxidant can scavenge the free radical and detoxify it. One of the potential plant developed as natural antioxidant is kelor (Moringa oleifera, Lamk). The aims of this research were to evaluate the activity of radical scaveng...
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[Yogyakarta] : Universitas Gadjah Mada
2014
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id-ugm-repo.1280682016-03-04T07:53:19Z https://repository.ugm.ac.id/128068/ ISOLASI DAN IDENTIFIKASI SENYAWA PENANGKAP RADIKAL 2,2-DIFENIL-1-PIKRILHIDRAZIL DALAM DAUN KELOR (Moringa oleifera, Lamk.) , BETA RIA ERIKA MARITA DELLIMA , Prof. Dr. Sugeng Riyanto, M.S., Apt ETD Free radical is suspected as mediator of various degenerative diseases. Antioxidant can scavenge the free radical and detoxify it. One of the potential plant developed as natural antioxidant is kelor (Moringa oleifera, Lamk). The aims of this research were to evaluate the activity of radical scavenging of 2,2- diphenyl-1-picrylhydrazyl (DPPH), the contents of phenolic total and flavonoid total of kelor leaves extract and its fractions and to isolate the active component responsible for DPPH radical scavenging activity. Dry powder of kelor leaves was macerated using ethanol 80%. Macerate was concentrated using rotary evaporator and called as ethanol extract of kelor leaves. The extract was partitioned using n-hexane, ethyl acetate, and water. The result of the partition was then concentrated in order to get n-hexane, ethyl acetate and water extracts. All kelor leaves extract was determined for its activity of radical scavenging of DPPH, the contents of total phenolic and total flavonoid by spectrophotometry. The most active extract (ethyl acetate extract) was subsequently fractionated using vacuum liquid chromatography with stationary phase of Merck gel silica 1.07734.1000 sized 0.063-0.200 and the mobile phase consisted of n-hexane, chloroform, ethyl acetate, and methanol in various composition. The fractionation of ethyl acetate extract of kelor leaves yielded 12 fractions. Fraction number 12, as the most active fraction of free radical scavenger, was then hydrolyzed and continued with isolation process using column chromatography with stationary phase of Merck gel silica 1.09385.1000 sized 0.040-0.063 with the mobile phase consisted of chloroform, ethyl acetate, and methanol in various composition. Yellow isolate on effluent 35-38 was tested for its purity and identified using UV spectrophotometry, high performance liquid chromatography (HPLC) photodiode array detector, infrared (IR) spectrophotometry, and mass spectrometry. The most active fraction (fraction no. 12) had IC50 value of 15.02 μg/mL, while the contents of total phenolic and total flavonoid were 11.14 % wt/wt gallic acid equivalent and 44.01 % wt/wt rutin equivalent. Identification using UV, IR and mass spectrometry showed that the isolate in effluent 35-38 contained quercetin aglycone. [Yogyakarta] : Universitas Gadjah Mada 2014 Thesis NonPeerReviewed , BETA RIA ERIKA MARITA DELLIMA and , Prof. Dr. Sugeng Riyanto, M.S., Apt (2014) ISOLASI DAN IDENTIFIKASI SENYAWA PENANGKAP RADIKAL 2,2-DIFENIL-1-PIKRILHIDRAZIL DALAM DAUN KELOR (Moringa oleifera, Lamk.). UNSPECIFIED thesis, UNSPECIFIED. http://etd.ugm.ac.id/index.php?mod=penelitian_detail&sub=PenelitianDetail&act=view&typ=html&buku_id=68397 |
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ETD , BETA RIA ERIKA MARITA DELLIMA , Prof. Dr. Sugeng Riyanto, M.S., Apt ISOLASI DAN IDENTIFIKASI SENYAWA PENANGKAP RADIKAL 2,2-DIFENIL-1-PIKRILHIDRAZIL DALAM DAUN KELOR (Moringa oleifera, Lamk.) |
| description |
Free radical is suspected as mediator of various degenerative diseases.
Antioxidant can scavenge the free radical and detoxify it. One of the potential
plant developed as natural antioxidant is kelor (Moringa oleifera, Lamk). The
aims of this research were to evaluate the activity of radical scavenging of 2,2-
diphenyl-1-picrylhydrazyl (DPPH), the contents of phenolic total and flavonoid
total of kelor leaves extract and its fractions and to isolate the active component
responsible for DPPH radical scavenging activity.
Dry powder of kelor leaves was macerated using ethanol 80%. Macerate
was concentrated using rotary evaporator and called as ethanol extract of kelor
leaves. The extract was partitioned using n-hexane, ethyl acetate, and water. The
result of the partition was then concentrated in order to get n-hexane, ethyl acetate
and water extracts. All kelor leaves extract was determined for its activity of
radical scavenging of DPPH, the contents of total phenolic and total flavonoid by
spectrophotometry. The most active extract (ethyl acetate extract) was
subsequently fractionated using vacuum liquid chromatography with stationary
phase of Merck gel silica 1.07734.1000 sized 0.063-0.200 and the mobile phase
consisted of n-hexane, chloroform, ethyl acetate, and methanol in various
composition. The fractionation of ethyl acetate extract of kelor leaves yielded 12
fractions. Fraction number 12, as the most active fraction of free radical
scavenger, was then hydrolyzed and continued with isolation process using
column chromatography with stationary phase of Merck gel silica 1.09385.1000
sized 0.040-0.063 with the mobile phase consisted of chloroform, ethyl acetate,
and methanol in various composition. Yellow isolate on effluent 35-38 was tested
for its purity and identified using UV spectrophotometry, high performance liquid
chromatography (HPLC) photodiode array detector, infrared (IR)
spectrophotometry, and mass spectrometry.
The most active fraction (fraction no. 12) had IC50 value of 15.02 μg/mL,
while the contents of total phenolic and total flavonoid were 11.14 % wt/wt gallic
acid equivalent and 44.01 % wt/wt rutin equivalent. Identification using UV, IR
and mass spectrometry showed that the isolate in effluent 35-38 contained
quercetin aglycone. |
| format |
Theses and Dissertations NonPeerReviewed |
| author |
, BETA RIA ERIKA MARITA DELLIMA , Prof. Dr. Sugeng Riyanto, M.S., Apt |
| author_facet |
, BETA RIA ERIKA MARITA DELLIMA , Prof. Dr. Sugeng Riyanto, M.S., Apt |
| author_sort |
, BETA RIA ERIKA MARITA DELLIMA |
| title |
ISOLASI DAN IDENTIFIKASI SENYAWA PENANGKAP RADIKAL 2,2-DIFENIL-1-PIKRILHIDRAZIL DALAM DAUN KELOR (Moringa oleifera, Lamk.) |
| title_short |
ISOLASI DAN IDENTIFIKASI SENYAWA PENANGKAP RADIKAL 2,2-DIFENIL-1-PIKRILHIDRAZIL DALAM DAUN KELOR (Moringa oleifera, Lamk.) |
| title_full |
ISOLASI DAN IDENTIFIKASI SENYAWA PENANGKAP RADIKAL 2,2-DIFENIL-1-PIKRILHIDRAZIL DALAM DAUN KELOR (Moringa oleifera, Lamk.) |
| title_fullStr |
ISOLASI DAN IDENTIFIKASI SENYAWA PENANGKAP RADIKAL 2,2-DIFENIL-1-PIKRILHIDRAZIL DALAM DAUN KELOR (Moringa oleifera, Lamk.) |
| title_full_unstemmed |
ISOLASI DAN IDENTIFIKASI SENYAWA PENANGKAP RADIKAL 2,2-DIFENIL-1-PIKRILHIDRAZIL DALAM DAUN KELOR (Moringa oleifera, Lamk.) |
| title_sort |
isolasi dan identifikasi senyawa penangkap radikal 2,2-difenil-1-pikrilhidrazil dalam daun kelor (moringa oleifera, lamk.) |
| publisher |
[Yogyakarta] : Universitas Gadjah Mada |
| publishDate |
2014 |
| url |
https://repository.ugm.ac.id/128068/ http://etd.ugm.ac.id/index.php?mod=penelitian_detail&sub=PenelitianDetail&act=view&typ=html&buku_id=68397 |
| _version_ |
1681232728387747840 |