Abstract
In this study, enzymatic hydrolysis of the holocellulose from Alnus hirsuta (Spach) Rupr. (8-14 yr's) was investigated using crude cellulase preparations of Trichoderma viride Pers. ex. Fr. SANK 16374. And conducted on the optimum condition of the treated substrate for saccharification. A strain of Trichoderma viride Pers. ex. Fr. SANK 16374 was found to be highly efficient for the cellulase productivity, especially in the submerged culture process. The culture medium used in this experiment was prepared from an extract of wheat bran consisting also of $KH_2PO_410$, $(NH_4)_2$ $SO_4$ 3, $NaNO_3$ 3, and $MgSO_4$ $7H_2O$ 0.5g/l. Cellulose powder (Toyo filter paper, 60 mesh) was found to be an importent factar for inducing the cellulase formation. And the cellulase produced in the culture fluid was salted out quantitatively by the use of ammonium sulfate (Fig. 1) Reducing sugar was determined by the Dinitrosalicylic acid (DNS) method, using reagents prepared according to the method of Sumner (1925). The results obtained were summerized as follows; 1. The method of delignification were treated by the Peracetic acid (PA) method, according to the method of Toyama (1970). The yield of holocellulose were decreased in accordance with increasing concentration of Peracetic acid solution; delignification of Alnus hirsuta Rupr. with 20% Peracetic acid was satisfied for 48 hours and 40%~60% peracetic acid was satisfied for 24 hrs: 2. The substrate (holocellulose) was changed easely into fine powder with enzymatic hydrolysis and cellulase exhibits optimum activity on the reducing sugar formation from substrate at the range of 60-100 mesh. 3. The reducing sugar formation increased in accordance with increasing dry temperature on holocellulose substrate was found to be $190{\pm}5^{\circ}C$. 4. The optimal heat treated time of holocellulose substrate was found to be 45 min. for the reducing sugar formation showed the best products. The reducing sugar formation did not show statisticaly significent diflerences at 5% levels by heat treated time for 45 min. and 60 min.
Trichoderma viride 16374호(號) Cellulase에 의(依)한 목재가수분해(木材加水分解)에 관(關)한 연구(硏究)로서 재료(材料)는 산오리나무재(材)를 사용(使用)하였다. 효소생산(酵素生産)은 액체(液體) 진탕배양법(振盪培養法)에 의(依)하였다. 즉(即) 밀기울 추출액(抽出液)에 Pulp분말(粉末)(Toyo여지(濾紙) 60 mesh) 10, $KH_2PO_410$, $(NH_4)_2$ $SO_4$ 3, $NaNO_3$ 3, $MgSO_4$ $7H_2O$ 0.5g/1을 가(加)하였다. 이와 같이 하여 진탕배양(振盪培養)한 후(後) 배양액(培養液)을 취(取)하여 유안포화도(硫安飽和度)에 의(依)한 염석조효소액(鹽析粗酵素液)을 만들었다. 환원당정량(還元糖定量)은 DNS법(法)에 의(依)하였다. (1) 탈(脫)리그닌은 외산(外山)(1970)의 과초산법(過醋酸法)에 의(依)하였다. 여기서 과초산(過醋酸)의 농도(濃度)가 높을수록 단기간(短期間)에 Pulp수율(收率)은 감소(減少)하였다. 즉(即) 20% 과초산액(過醋酸液)으로 처리(處理)한 시료(試料)는 48시간(時間)에, 40% 및 6% 과초산액(過醋酸液)으로 처리(處理)한 시료(試料)는 24시간(時間)이면 충분(充分)한 탈(脫)리그닌이되었다. (2) 기질(基質)은 징세(徵細)할수록 효소(酵素)에 의(依)한 가수분해(加水分解)가 용이(容易)하였으며 환원당생성(還元糖生成)에 적합(適合)한 기질(基質)의 크기는 60-100mesh로 나타났다. (3) 기질(基質)의 건조온도(乾燥溫度)는 높을수록 환원당생성량(還元糖生成量)이 증가(增加)하였으며, 여기서는 건조온도(乾燥溫度)가 $190{\pm}5^{\circ}C$에서 가장 많은 당생성(糖生成)이 나타났다. (4) 기질(基質)의 열처리시간(熱處理時間)이 가장 적당한 것은 45분(分)으로 나타났다. 그리고 45분(分)과 60분간(分間) 열처리(熱處理)한 기질(基質)의 환원당(還元糖) 생성량(生成量)에는 유의차(有意差)가 인정(認定)되지 않았다.