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KEYWORDS 

Shelf-life; smoked herring; 

volatile compounds; 

microbiological analyses. 
 
 

PAGES 

9 – 14  

 
 

REFERENCES 

Vol. 1 No. 1 (2014) 

 

 

ARTICLE HISTORY 

Submitted: November 04, 2013 

Revised: January 29, 2014 

Accepted: February 03, 2014 

Published: February 10, 2014 

 
 

CORRESPONDING AUTHOR 

Cristian Bernardi, 

Laboratory of Food Inspection, 

Department of Health, Animal 

Science and Food Safety - 

Università degli Studi di Milano 

 

Via Celoria, 1 – 20133 

 Milan, Italy 
 

e-mail: cristian.bernardi@unimi.it 

phone: +39 02 50318506 

fax: +39 02 50318501 

 
 

JOURNAL HOME PAGE 

riviste.unimi.it/index.php/haf 

 
 

A case study: shelf-life of 

smoked herring fillets by 

volatile compounds 

analysis. 

 

Cristian Bernardi
1*

, Erica Tirloni and Patrizia Cattaneo 

 

1
 Laboratory of Food Inspection, Department of Health, Animal Science 

and Food Safety, Università degli Studi di Milano. 

 

 

ABSTRACT. 

Two different products of vacuum packed cold smoked herrings were 

analyzed at time intervals in order to evaluate the efficiency of the 

processing and product stability. Microbiological total counts, lactic acid 

bacteria, total coliforms, pH, water activity, water content, salt content 

(WPS) were determined. Differences in hygienic conditions and salt content 

were found. Principal components analysis (PCA) of volatile compounds 

determined by GC-MS analysis allowed the differentiation of the processing. 

 



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1 Introduction 

The more widespread smoked herrings marketed in Italy are beheaded with skin, vacuum 

packaged, silver and golden types; less frequent are skinned fillets, softer and with a milder 

taste, vacuum packaged, which meet more with the liking of the modern consumer. The cold 

smoked herring is at the limit of the group of the lightly preserved seafood (Huss, 1994), 

comprising products with low salt level (<6% NaCl-Water Phase Salt WPS), preservatives or 

smoke, pH value >5, mainly vacuum packaged, requiring refrigeration temperatures and typically 

consumed as ready-to-eat without heat treatment. 

The process must allow the survival of an adequate number of spoilage organisms, which 

have the important role to compete with the growth and toxin formation of C. botulinum type E 

and non-proteolytic types B and F (FDA, 2001a).  

The control measures of potential hazards are based mainly on salt control (nitrite addition 

is not allowed by EC regulation in these products), on control of exposition to temperatures that 

favour C. botulinum throughout the processing steps, on maintenance at refrigeration 

temperatures of the final products. With regard to this, US HACCP regulations suggest a critical 

limit for vacuum packaged cold smoked products of at least 3.5 % NaCl –WPS at  4.4°C, allowing 

for short time periods temperatures up to 10°C (FDA, 2001b). 

The purpose of this investigation was to answer an importer’s request, that was to verify the 

established shelf-life of smoked vacuum packed herring fillets of a new producer (product A). 

With this aim traditional analytical techniques and SPME headspace-gas chromatography-mass 

spectrometry were applied comparing product A to a traditional one (B) on the furnished 

packets. 

 

 

2 Materials and Methods 

A total of 18 packets of smoked herring fillets, peeled and vacuum packed of two different 

producers were compared (10 of producer A, 8 of B). The packages were stored at 0-2°C for the 

whole period of the trial. Analyses were performed as described in Bernardi et al., 2009. Water 

activity (aW), water content, NaCl–WPS were performed in quadruplicate. The enumeration of 

Total Psychrotrophic Count (TPC), Lactic Acid Bacteria (LAB), total coliforms, pH and SPME GC-

MS analyses were performed at time intervals in duplicate. Volatile compounds were tentatively 

identified by matching mass spectral data with the Wiley and NIST reference libraries of 

standard compounds. The identification was confirmed by comparison of the retention times 

and mass spectra (MS) with available authentic standards (AS). Semi-quantification of the 

compounds was based on arbitrary units of peak area counts divided by 105. 

 

 

3 Statistical analysis  

Principal component analysis (PCA) and statistical analysis were performed by the SPSS 

package version 9.0 (SPSS Italia, Bologna). 



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4 Results and discussion 

WPS rate was amply above the 3.5 % NaCl-WPS; in product B, salt content was more variable; 

aW was similar in both, but more variable in product A, allowing to consider safe both products. 

Product A had at the arrival (27
th

 days from production) a very high TPC (5.74 Log CFU/g), 

afterwards TPC decreased and LAB counts overcame 7 Log CFU/g, but without causing 

detectable olfactory deterioration of flavour. 

Product B showed lower TPC and LAB than A (<3.70 and 5.78 Log CFU/g, respectively at 9
th

 

days). Total coliforms were under the limit of detection (<2 Log CFU/g) both in A and B (table 

n.1). 

In product B forty-five peaks were determined and identified by GC-MS. Particularly, in 

product B benzaldehyde and furfural and small quantities of propionaldehyde and hexanal were 

present, while absent in A. Phenol was present in both, without significant differences. Acetic 

acid was found more in product B. Dimethyl sulfoxide and dimethyl sulphide were more 

represented in A than in B. As a whole, product B showed an aromatic profile more complex and 

rich in qualitatively superior compounds, while product A showed a very little articulate profile. 

In figure n. 1 the analysed samples and the identified variables (volatile compounds) are 

represented in the space described by the two principal components, the first component 

explaining 78.3% variability among data, the second component explaining 9.2% variability. 

Samples are clearly distinguished in two groups, coinciding with A and B productions. The 

second component allows to distinguish product A on 27
th

 day from the subsequent samples. 

On the “best before” date, product A had an initial softening with presence of fluid material 

in the pack, without other sensorial changes; product B maintained a better firmness, also for a 

lesser water content. The bacterial count at the first sampling of A was high, indicating bad 

hygienic condition, while the product B was hygienically better at about the same storage time. 

Product A had a higher salt content; this was a negative aspect, not only from a nutritional 

point of view, but also for the consumer’s present preferences; its WPS ratio allowed the same 

stability of the product B although a higher water content. WPS more than 6% puts both 

products at the limit between lightly preserved and semi-preserved seafood (Huss, 1994).  

The obtained results allowed to assume a different processing technology: brine salting for 

A, due to the high water level and the uniform salt content of the fillets, while for B a dry salting 

process with purging was probable, because of a considerably lower water content and a higher 

variability in the salt concentration (Coefficient of Variation 13.8%). 

In the verified conditions, the shelf life of product A is to be stated up to 4 weeks instead a 

“best before” date of 45 days; microbiological parameters of B were stable for the whole period 

of the trail. The exclusive presence in the product B of benzaldehyde and furfural, aldehydes 

known for giving a strong taste of smoke, confirmed the perception of a more typical aroma of 

the herring B. 

The clear finding of dimethyl sulfoxide and dimethyl sulphide only in the product A, well 

match with the microbial condition of A; these sulphur compounds may be the expression of 

bacterial activity besides of ripening (Triqui, 1995). 

 

 



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Table 1. Conservation parameters. 

Sample A B 

 m M Mean SD CV m M Mean SD CV 

aw 0.923 0.966 0.943 0.014 0.36 0.940 0.949 0.945 0.004 1.48 

Water content % 72.25 75.18 74.12 1.12 1.51 60.39 66.73 63.26 2.62 4.13 

Salt % 5.25 5.59 5.43 0.14 2.64 3.76 4.85 4.38 0.53 12.13 

WPS % 6.57 6.92 6.83 1.46 2.14 5.62 7.43 6.48 0.90 13.84 

 

Microbiological 

analyses 
A B 

day 27 45 49 55 60 9 26 30 41 

TPC 
(Log CFU/g) 

5.74 <4.70 <3.70 <3.70 <3.70 <3.70 <3.70 <3.70 <3.70 

LAB 
(Log CFU/g) 

6.78 7.63 <4.70 7.38 7.30 5.78 6.48 6.54 6.90 

Coliforms 
(Log CFU/g) 

<2.00 <2.00 <2.00 <2.00 <2.00 <2.00 <2.00 <2.00 <2.00 

Legend: 

m = minimum value 

M = maximum value 

CV = coefficient of variation 

TPC= Total Psychrotrophic Count 

LAB=Lactic Acid Bacteria 

 

 

5 Conclusions 

The results related to the study of the volatile fraction confirmed what deduced by the more 

traditional analyses: in spite of the close outward likeness between the two products, their 

processing technologies were very different, resulting in distinct products as regards shelf life 

and quality. The reported case is an example of the result of the delocalization, due to 

economical reasons, of food processing in countries applying less advanced or less consolidated 

technologies or procedures with inferior process standard. 



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Figure 1. Biplot of principal component scores and factor loadings from principal component 

analysis applied to volatile compounds of product A (scores L) and product B (scores D). 

Volatile compounds identified in smoked herring (Clupea harengus) by GC-MS: 1) 2-pentene; 2) 

heptane; 3) dimehyil sulphide; 4) methyl-cyclo-hexan; 5) propanal; 6) furan; 7) propanone; 8) 

methyl acetate; 9) 2-methyl-furan; 10) ethyl acetate; 11) 2-butanone; 12) 3-methyl-butanale; 13) 

ethanol; 14)benzene; 15) 2-ethyl-furan; 16) branched hydrocarbon; 17) 2-pentanone; 19) 

chloroform; 20) hexanal; 21) p-xylene; 22) cyclopentanone; 23) 2-methyl-cyclo-pentanone; 24) 3-

methyl-cyclo-pentanone; 25) pyrazine; 26) cyclohexanone; 27) acetoin; 28) 2-methyl-2cyclo-

pentenone; 29) 3-furaldehyde; 30) acetic acid; 31) 2-furaldehyde; 32) acetyl-furan; 33) 

benzenaldehyde; 34) propanoic acid; 35) dimethylsulfoxide; 36) 5-metil 2-furaldehide; 38) 

gamma-butyrolactone; 39) butanoic acid; 40) 3,4-dimethyl-3-penten-2-one; 41) 5-metil-2(5H)-

furanone 44) 2- pyranone; 45) 2-methoxy-phenol; 46) guaiacol; 47) phenol; 50) 2-furanone. 

 

 

 

  



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References 

Bernardi, C., Ripamonti, B., Campagnoli, A., Stella, S., Cattaneo, P., 2009. Shelf-life of vacuum 

packed Alaskan, Scottish and Norwegian cold-smoked salmon available on the Italian 

market. International Journal of Food Science and Technology. 44, 2538-2546. 

FDA, Center for Food Safety & Applied Nutrition, 2001a. Fish and fisheries products hazards and 

controls guidance. Third Edition, June. 

FDA, Center for Food Safety and Applied Nutrition, 2001b. Processing Parameters Needed to 

Control Pathogens in Cold-smoked Fish. Supplement to Journal of Food Science. 66, (7), S-

1133. 

Huss, H.H., 1994. Assurance of seafood quality. FAO Fisheries Technical Paper. 334, FAO, Rome, 

Italy. 

Triqui, R., Reineccius, G.A., 1995. Changes in flavour profiles with ripening of anchovy (Engraulis 

encrasicholus). Journal of Agriculture and Food Chemistry. 43, 1883–1889.