BIOTROPIA NO


BIOTROPIA NO. 16, 2001 : 28 - 38 

CHARACTERIZATION OF MALAYSIAN WILD BANANAS BASED 
ON ANTHOCYANINS 

MUHAMMAD ASIF JAVED*, MAK. CHAI AND ROFINA YASMIN OTHMAN 

Division of Genetics, Institute of Biological Sciences, University of Malaya 
50603 Kuala Lumpur, Malaysia 

ABSTRACT 

The male buds of 16 Musa species (Musaceae) populations were investigated by HPLC for the 
occurrence of anthocyanins. The investigation was based on the presence of 6 anthocyanins. The 16 Musa 
samples could be classified into three distinct species i.e. Musa acuminata, Musa violascens and Musa 
balbisiana. Musa acuminata could be divided into two subspecies : malaccensis (lowland) and tmncata 
(highland) according to their constituents and content of major anthocyanins. No variation was observed in 
the composition of the anthocyanins of Kedah type ssp. siamea and Selangor types ssp. malaccensis. The 
classification of M. acuminata into two subspecies based on anthocyanin data further supported the current 
taxonomic grouping of the species. 

Key words: Musa acuminata/Musa violascens/Musa balbisiana/Musaceae /HPLC /chemotaxonomy 

INTRODUCTION 

The classification of the genus Musa as proposed by Cheesman (1947) is the 
only one which accords satisfactorily with the known taxonomic and cytogenetic 
facts. Of the four named sections, Eumusa is the best known partly because the 
plants are hardy and fairly easy to grow whereas the Callimusa is the least known 
section. Section Eumusa is the most important as the progenitor of all cultivated 
bananas. Musa acuminata (AA) and Musa balbisiana (BB) belong to this section. 
Among the cultivated bananas, different cultivars are classified according to their 
genomic constitution and ploidy level. 

Malaysia is one of the centers of diversity of wild and cultivated bananas. 
Simmonds (1955) reported four species from the Malaysian peninsula. The two 
species Musa violascens and Musa gracilis are ornamental wild bananas whereas 
Musa acuminata and Musa balbisiana are the two most important species of the 
genus Musa. Musa acuminata is the most variable species of the two in Malaysia 
being the progenitors of several local diploid and triploid banana cultivars. Three 
different subspecies of Musa acuminata suggested (Simmonds 1955) were ssp. 
malaccensis (Selangor), truncata (Cameron highland) and siamea (Kedah). This 
classification was questioned by Hari (1968) and then later on Shepherd (1988) 
based on chromosomal translocations. Therefore, the nomenclature of local wild 
Musa species has been complicated by taxonomic revisions. Recent renewed interest 

*   Corresponding Author: e-mail. J95asit@umcsd.um.edu.my 
rocketmail. Asif_Javed@rocketmail.com 

28 



BIOTROPIA NO. 16, 2001 

in the utilization of wild banana sources had further elucidated the need to 
characterize different wild Musa species in Malaysia. 

Anthocyanins constitute the most important group of plant pigments. In 70 
species of 33 families of angiosperms, they were found in membrane-bounded 
anthocyanoplasts located within the main cell vacuole. Apart from contributing 
cyanic color to flower and fruits, the pigments also play an important role during 
pollination, and are of great economic and genetic importance. Previous surveys of 
anthocyanins in the bracts of banana have been reviewed (Simmonds 1954 b,c; 
Horry and Jay 1988 a,b). The distribution of various anthocyanidins among different 
banana cultivars gave good support to the taxonomic ordering within the genus 
(Horry and Jay 1988a,b). 

The present study described the relationship between different wild bananas of 
Malaysian origin based on the distribution of anthocyanins. 

MATERIALS AND METHODS 

Sample Collection 

Wild Musa species samples were collected from different parts of Peninsular 
Malaysia. The types and number of samples collected and their locations are shown in 
Table 1. Fourteen populations of wild Musa acuminata were sampled. Samples of 
Musa violascens and Musa balbisiana were also selected for comparative studies. 
Ten suckers each of Musa acuminata, Musa violascens and Musa balbisiana were 
collected from different mother plants and these were planted in the university farm 
for evaluation. Suckers were planted in holes of 30-40 cm deep, spaced at 2 m x 2 m. 
At planting, organic compost was applied in the holes. Weeding was done 
manually. 

Anthocyanin Extraction 

Variation in anthocyanin pigments was studied from male buds collected from 
16 samples (Table 1). Each banana sample consisted of three male buds as three 
replicates. The outermost male bracts were used for anthocyanin extraction by 
grinding 4-5 g of bracts to powder form in liquid nitrogen. Anthocyanin pigments 
were then extracted by boiling the powder in 40 ml of MeOH - EtOH (1:1) for 40 
minutes. Crude extracts were concentrated to 5 ml, and filtered through glass wool 
(Horry and Jay 1988a). Filtrates were stored at -70°C till used for thin layer 
chromatography (TLC) and high pressure liquid chromatography (HPLC). 

TLC and HPLC analysis 

Thin layer chromatography (TLC) was carried out on 0.1 mm cellulose plates 
(Merck. 1.05716. 20x20 cm). Development was accomplished with solvent mixtures 
prepared from analytical grades of hydrochloric acid, formic acid and deionized dis- 

29 



Characterization of Malaysian wild bananas – Muhammad Asif javed et al 
 
 
Table 1. Samples of  wild Musa species 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
``tilled water. Two solvent systems used for TLC were : a. System I. Cone. HC1 -
Formic acid - Water (24.9:23.7: 51.4), b. System II. Cone. HC1 - Formic acid -
Water (7.1:31.4:61.5). 

Developing tanks were lined with heavy grade filter paper and allowed to 
equilibrate overnight prior to use. TLC plates were kept at 80°C overnight. A base 
line was drawn on the loading end and a 1-2 ul of concentrated anthocyanin 
solutions were loaded. There were 10 samples loaded on each plate. Rf values taken 
for each pigment according to their mobility on the TLC plate were calculated as 
follows; 

    Distance of migration substance  
Rf =  

Distance of migration of solvent front 

HPLC analysis of anthocyanin pigments was carried out on a Millipore 
Waters™ liquid chromatograph equipped with a variable wavelength Waters™ 486 
detector, Waters™ 600 controller and Waters™ 717 plus auto-sampler was used. 
Anthocyanin pigments separation was carried out using reverse phase C - 18, 
Inertsil ODS -2 (4.6 x 1.6 mm) 5 urn column (Horry and Jay 1988a). 

HPLC was run according to Horry and Jay (1988a), with slight modifications. 
Two solvents used were 5% Formic acid and absolute methanol (5:95, v/v). 
Concentrated anthocyanin extracts were diluted ten times with 0.1N HC1, and 
filtered just before injection. Flow rate was maintained at 0.80 ml/min with an 
injection volume of 20 ul. Detection was observed at 514 nm or 240 to 600 nm with 
scanning detector for spectral identification of the peaks. The aglycone moiety of the 

30 



BIOTROPIA NO. 16, 2001 

anthocyanin for each HPLC peak was identified according to the maxima of 
absorbance in the visible range (compounds 3, 6, 8: X max vis = 530, 535, 535 nm; 
compounds 4, 5, 7: A. max vjs = 520, 522, 522 nm) and to their retention times whereas 
glycosidic pattern was determined by TLC. The composition of the two solvents, 
flow rate and time are given in Table 2. 

Table 2. Method used for anthocyanin separation by HPLC system (Horry and Jay 1988a) 
 
 
 
 
 
 
 

 
 
 
The peaks showing different anthocyanin pigments (delphinidin, derivative of 

cyanidin, cyanidin, petunidin, peonidin and malvidin) were used for sample com-
parison. 

Chemometric Analysis 

HPLC data from 16 Musa samples were subjected to cluster analysis and 
principal component analysis (PCA) using SPSS statistic program (SPSS, Inc.). 
Relative amounts of the anthocyanins expressed by percentages were used as an 
input matrix. 

RESULTS 

Anthocyanins were extracted from the outer most bracts tested through thin 
layer chromatography (TLC) followed by high pressure liquid chromatography 
(HPLC). Different pigments separated by HPLC were determined according to 
increasing retention times, and only six compounds were identified. The absence of a 
shoulder around 330 nm indicated the absence of acylation. The presence of a 
shoulder in the visible spectrum at 440 nm and the Rf values obtained on TLC 
indicated the presence of 3- rutinosides as also reported by Horry and Jay (1988a). 

Thin layer chromatography on 0.1 mm cellulose layer plates clearly showed the 
separation of different anthocyanin pigments. Rf values obtained on TLC indicated 
the presence of 3- rutinosides namely 3-O-rutinosyldelphinidin, 3-O-rutinosyl-
cyanidin, 3-O-rutinosylpeonidin, and 3-O-rutinosylmalvidin (Table 3). 

High pressure liquid chromatography (HPLC) of anthocyanins resolved Musa 
samples into a maximum of nine peaks. The peaks appearing between 10 to 21 
minutes were the six peaks representing the six anthocyanins according to their 
retention times (Horry and Jay 1988a,b). 

31 



Characterization of Malaysian wild bananas - Muhammad Asif Javed et al 

The same sample injected three times did not show any difference in the 
chromatograms showing the stability of the system and the anthocyanin pigments. 
Similarly, anthocyanin components extracted from the three outermost bracts from 
the same male bud did not show any difference in the number of anthocyanin 
components. The color of the bract in the male inflorescence progressively vanishes 
from the outside bract (bract 1, the oldest) to the inner bracts. It was observed that 
the relative distribution of the anthocyanin pattern is stable from the outer bracts to 
the inner bracts. 

Extracts from Musa acuminata accessions, BC2 and Gala were analyzed and 
the results are presented in Table 4. Six previously reported anthocyanins were 
observed to be piesent in different combinations and percentages among all the 
samples studied except Flava (Table 4). 

Table 3. Anthocyanin of banana bracts separated through TLC by using two different solvent systems 

 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
32 



BIOTROPIA NO. 16,2001 

The data matrix of relative amounts of floral anthocyanins expressed by 
percentages for Musa samples (Table 4) was then subjected to cluster and principal 
component analysis (PCA). Cluster analysis was conducted by using Ward's method 
with squared euclidean distance (Fig 1). Four principal components with eigenvalues 
more than 1.0 were obtained, which could explain 99.89% for the total variation in 
the data matrix. Thus all samples were grouped into four based on cluster and 
principal component analysis (Table 5). 

Rescaled Distance Cluster Combined 

 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
Figure  1. Cluster analysis of Musa accessions based on anthocyanins using Ward's method. All Musa 

acuminata accessions were grouped into two major clusters except for the sample Flava. The 
highland banana BC3 was well separated from other Musa acuminata accessions. Similarly, 
Gala (Musa balbisiana) and BC2 (Musa violascens) were also well separated. 

 
 
 
 

33 



Characterization of Malaysian wild bananas - Muhammad Asif Javed et al 

Gala was completely separated from the Musa acuminata and Musa violascens 
by larger values in the score for third PC (Table 5), and is characterized by the larger 
accumulation of cyanidin (84.63%) followed by cyanidin derivative (Table 4). 
Factor loadings of pigments cyanidin and cyanidin derivative for the third PC were 
also great (Table 6). 

Highland Musa acuminata sample (BC3) was completely separated from other 
samples of the species gaining the highest score for the second PC (Table 5), for 
which factor loadings of pigment petunidin were great (Table 6), whereas the 
cyanidin derivative was also accumulated in the highest percentage compared to 
other accessions of M acuminata samples. However, this sample showed the lowest 
peonidin compared to other samples of the same species. 

Table 5. Principal component scores of Musa samples 

 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
Table 6. Factor loadings of respective pigments exiting in Musa species to principal components 
 
 
 
 
 
 
 
 
 
 

 
 
 
34 



BIOTROPIA NO. 16, 2001 

Musa violascens (BC2) showed a very different chemotype and a number of 
peaks produced varied from other two species samples greatly. The anthocyanins 
detected in the other two species were present in a very small percentage. Similarly, 
Musa acuminata sample Flava was observed with a very small percentage of the six 
anthocyanins detected. 

Twelve samples were classified into first group gaining the largest scores for 
first principal component (Table 5), for which factor loadings of peonidin, cyanidin 
and malvidin were great (Table 6), whose anthocyanin composition of the bracts 
seems to be the standard of the Musa acuminata samples. The only variation 
observed among these samples was the ratio of peonidin and malvidin. Different 
from the highland banana samples with a large accumulation of peonidin whereas, 
cyanidin derivative and petunidin were present in a very low percentage (Table 4). 

As shown in Fig (1) and Table (5), three groups of Musa acuminata were 
readily distinguishable. Flava diverges from other two groups of samples by'the 
absence of anthocyanins, as it had yellow color bracts i.e. acyanic bracts. Highland 
banana sample BC3, had a very distinct deep chocolate brown color of the male 
bracts, and was characterized with accumulation of the simple anthocyanins in this 
subspecies, whose total composition could be described as 3 - rutinosides of 
cyanidin derivative (Cyd), 3 - rutinosides of petunidin (Pt) (Table 4). These 
anthocyanins were mainly present in this sample. However, a low percentage of 
peonidin was detected. The remaining Musa acuminata accessions belonging to 
lowlands of Malaysia showed similar anthocyanins and their bract color ranged from 
red and purple. Similarly, all Musa acuminata accessions suggested a very high 
ability of methylation of anthocyanidins compared to Gala (M. balbisiana). 

DISCUSSIONS 

Many cytotaxonomists have argued that a unique chemical feature should merit 
the same importance as an unusual leaf shape or an odd chromosome number in 
determining plant relationships. They have shown that chemical characters correlate in 
genetic surveys satisfactorily with one or more biological characters. Harborne 
(1967) made a survey of flavonoid pigments in 45% of the genera in the family 
Gesneriaceae against the classification proposed based on morphological grounds. 
The differences at the subfamily level indicated a correlation between anthocyanin 
chemistry and plant geography. 

Anthocyanin components were found to be very stable and the chromatograms 
obtained were highly reproducible under the same conditions. Although the yield of 
anthyocyanins in Musa accessions may vary, the qualitative aspect of it remains 
relatively consistent, thus making them good taxonomic characters. More than nine 
peaks were observed in most of the samples, indicating that at least similar number of 
components were present. However, in the present study only six components 
were recognized following Horry and Jay (1988 a,b). From the chromatograms, all 
the Musa species can be identified. Musa acuminata accessions were characterized 

35 



Characterization of Malaysiar, wild bananas - Muhammad Asif Javed el al 

with partially methylated anthocyanins based on cyanidin - delphinidin mixtures i.e. 
mixtures of cyanidin, peonidin, delphinidin, petunidin and malvidin in different 
proportions. Flava, a yellow bracted accession, did not show significant amount of 
anthocyanins. Simmonds (1954) reported that Musajlava Ridl. from Malaysia was 
merely a yellow bracted form of Musa acuminata and the yellowness was due a 
single recessive gene and Flava was a good example of acyanic bracts (bracts 
without anthocyanins). Musa violascens was observed with a very different 
chromatogram than the other two and it showed a very little amount of six 
anthocyanins as observed in remaining species. The anthocyanin variation observed in 
this species could also be related to the light pink bract color compared to the red 
purple color observed in other species. Anthocyanin variation among these species 
was further suggested by their different pollinators. Musa violascens were reported 
to be bird pollinated whereas M. acuminata and M. balbisiana flowers were 
pollinated by bats (Simmonds 1962; Argent 1976). 

Horry and Jay (1988 a, b) described a schematic sequence for anthocyanin 
biosynthesis in Musa. They described that cyanidin is the first and simplest element in 
a sequence of hydroxylations whereas methylations ending at malvidin. Cyanidin or 
peonidin always occur, suggesting that cyanidin is an obligatory intermediate. We 
have observed high levels of cyanidin and peonidin in all Musa acuminata 
accessions except for the highland banana form BC3. BC3 was observed to have a 
very low level of peonidin whereas a new compound Cyd (cyanidin derivative) was 
deposited in high percentage compared to all other accessions. This compound was 
also reported by Horry and Jay (1988a, b) in Musa balbisiana and suggested a 
different biochemical pathway. It is found to be an interesting marker for highland 
banana forms, therefore, it merits further characterization. A similar situation was 
observed for petunidin, which was accumulated in a very high percentage in BC3. 
Horry and Jay (1988b) suggested that a low level of petunidin and the fact that it 
never accumulates without malvidin, leads to the assumption of O-methylations. 
These two compounds were observed in high percentage in all lowland banana 
samples except in BC3. 

In terms of evolutionary significance of anthocyanins, there is a trend for 
delphinidin to be replaced by cyanidin, which is considered to be the most primitive 
pigment. Therefore, O-methylation represents an advanced feature in comparison 
with simple hydroxylation (Harborne 1977). All lowland Musa acuminata acces-
sions were observed with low levels of petunidin compared to the high percentage of 
malvidin, suggesting an advanced feature of anthocyanins whereas it was different in 
highland banana accession showing a high percentage of petunidin. Simmonds 
(1962); Horry and Jay (1988a,b) suggested that chemotype of Musa balbisiana is 
fairly unique and possesses no "advanced" anthocyanin forms and that environ-
mental constraints were not so extreme that specialized biochemical pathways were 
needed to be developed in the evolution of this species. On the other hand, Musa 
acuminata was found to possess a broad range of chemotypes, indicating the 
presence of a more diversified metabolism. This suggests that Musa acuminata has 
undergone more evolutionary changes than Musa balbisiana. 

36 



BIOTROPIA NO. 16, 2001 

Cluster analysis and principal component analysis (PCA) produced five 
groupings in Musa acuminata accessions based on anthocyanins. The highland 
banana BC3 showed completely different anthocyanin patterns and was well sepa-
rated from the remaining accessions. It was also observed to be morphologically 
distinct. All lowland Musa acuminata accessions showed variation mainly in the 
proportion of the peonidin and malvidin. Malvidin was predominant in RI, IPTJ, 
BD1, BC1, Segun, Sintok, Rangis, and Perak whereas peonidin in Kra, BD2, PPC 
and J-4, respectively. The discrimination found among accessions, therefore, was 
mainly due to the ratios of these two anthocyanins whereas overall anthocyanin 
distribution was found similar among these accessions and the mean chemotype 
proceeded from a simple readjustment of the metabolic balance between methylated 
anthocyanins (Horry and Jay 1988a). 

The relationship revealed by the anthocyanin fingerprints could be compared 
with the geographical distribution and origin of these accessions. Musa acuminata 
accessions were collected from lowlands and highlands. A large variation in the 
anthocyanin composition was observed for the highland banana form (ssp. truncatd) 
compared to lowland samples. Northern (ssp. siamea) and central Malayan (ssp. 
malaccensis) region samples were observed with similar anthocyanin compositions. 
Therefore, the geographical origin of lowland accessions had little effect upon the 
anthocyanins metabolism. Whereas the highland banana was different in ecology 
and geography and also showed distinct anthocyanin pattern. 

Anthocyanin data further supported the two groupings of the Musa acuminata 
i.e. lowland (ssp. malaccensis) and highland (ssp. truncatd) as suggested by Hari 
(1968) and Shepherd (1988). 

ACKNOWLEDGEMENTS 

The work was supported by a grant from the Ministry of Science and 
Technology and Environment, Malaysia. We also would like to thank Mr. Gopal 
Krishnen and Mr. Asokan for their kind help in running the HPLC system analysis. 

REFERENCES 

Anderson, O. M. and G. W. Francis. 1985. Simultaneous analysis of anthocyanins and anthocyanidins on 
Cellulose thin layers. J. Chromatography. 318,450-454. 

Argent, G. C. G. 1976. The Wild Bananas of Papua New Guineae. Notes of Royal Botanical Garden, 
Edinburgh 35: 77-114. 

Cheesman, E. E. 1947. Classification of the Bananas. Kew Bull. 3, 11-28. 
Hari, P. C. 1968. Bract imbrication as a taxonomic character in Musa acuminata. Trop. Agric. Trinidad. 

Vol. 45, No. 2,99-108. 
Harborne, J.B. 1967. Comparative biochemistry of the flavonoids. Academic Press. London. 
Harborne, J. B. 1977. Flavonoids and the evolution of angiosperms. Biochem. Sys. Ecol. 5, 5-22 

37 



Characterization of Malaysian wild bananas - Muhammad Asif Javed et al 

Horry, J. P. and M. Jay. 1988a. Distribution of anthocyanins in wild and cultivated banana varieties. 
Phytochemistry. 27, 2667-2672. 

Horry, J. P. and M. Jay. 1988b. An evolutionary background of bananas as deduced from flavonoids 
diversification. In: (Jarret, R. L. ed.). Identification of Genetic Diversity in the genus Musa, 
INIBAP. Montpellier, France, p. 158-165. 

Shepherd, K. 1988. Observations on Musa taxonomy. In: (Jarret, R. L. ed.). Identification of Genetic 
Diversity in the genus Musa, INIBAP. Montpellier, France, p. 158-165. 

Simmonds, N. W. 1954b. Anthocyanins in bananas. Nature, 173,402. Simmonds, N. 
W. 1954c. Anthocyanins in banana. Ann. Bot. Lond. 18, 471-82. Simmonds, N. W. 
1955. Wild bananas in Malaya. Malayan Nature Journal. 10, 1-8. Simmonds, N. W. 
1962. The evolution of the bananas. London. UK. Longman. 

38